NIH Public Access: Author Manuscript
NIH Public Access: Author Manuscript
NIH Public Access: Author Manuscript
Author Manuscript
J Allergy Clin Immunol. Author manuscript; available in PMC 2010 August 18.
Abstract
The immune system has evolved to protect the host from a universe of pathogenic microbes that
are themselves constantly evolving. The immune system also helps the host eliminate toxic or
allergenic substances that enter through mucosal surfaces. Central to the immune systems ability
to mobilize a response to an invading pathogen, toxin or allergen is its ability to distinguish self
from non-self. The host uses both innate and adaptive mechanisms to detect and eliminate
pathogenic microbes. Both of these mechanisms include self-nonself discrimination. This
overview identifies key mechanisms used by the immune system to respond to invading microbes
and other exogenous threats and identifies settings in which disturbed immune function
exacerbates tissue injury.
Keywords
Adaptive immunity; atopy; B cell; complement; costimulation; inflammation; innate immunity;
superantigen; T cell; tolerance
Introduction
Humans and other mammals live in a world that is heavily populated by both pathogenic and
non-pathogenic microbes, and that contains a vast array of toxic or allergenic substances that
threaten normal homeostasis. The community of microbes includes both obligate pathogens,
and beneficial, commensal organisms, which the host must tolerate and hold in check in
order to support normal tissue and organ function. Pathogenic microbes possess a diverse
collection of mechanisms by which they replicate, spread and threaten normal host
functions. At the same time that the immune system is eliminating pathological microbes
and toxic or allergenic proteins, it must avoid responses that produce excessive damage of
self-tissues or that might eliminate beneficial, commensal microbes. Our environment
contains a huge range of pathogenic microbes and toxic substances that challenge the host
by a very broad selection of pathogenic mechanisms. It is not surprising, therefore, that the
immune system uses a complex array of protective mechanisms to control and usually
eliminate these organisms and toxins. A general feature of the immune system is that these
mechanisms rely on detecting structural features of the pathogen or toxin that mark it as
distinct from host cells. Such host-pathogen or host-toxin discrimination is essential to
permit the host to eliminate the threat without damaging its own tissues.
The mechanisms permitting recognition of microbial, toxic, or allergenic structures can be
broken down into two general categories: i) hard-wired responses that are encoded by genes
in the hosts germ line and that recognize molecular patterns shared both by many microbes
and toxins that are not present in the mammalian host; and ii) responses that are encoded by
gene elements that somatically rearrange to assemble antigen-binding molecules with
exquisite specificity for individual unique foreign structures. The first set of responses
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constitutes the innate immune response. Because the recognition molecules used by the
innate system are expressed broadly on a large number of cells, this system is poised to act
rapidly after an invading pathogen or toxin is encountered and thus constitutes the initial
host response. The second set of responses constitutes the adaptive immune response.
Because the adaptive system is composed of small numbers of cells with specificity for any
individual pathogen, toxin or allergen, the responding cells must proliferate after
encountering the antigen in order to attain sufficient numbers to mount an effective response
against the microbe or the toxin. Thus, the adaptive response generally expresses itself
temporally after the innate response in host defense. A key feature of the adaptive response
is that it produces long-lived cells that persist in an apparently dormant state, but that can reexpress effector functions rapidly after another encounter with their specific antigen. This
provides the adaptive response with the ability to manifest immune memory, permitting it to
contribute prominently to a more effective host response against specific pathogens or toxins
when they are encountered a second time, even decades after the initial sensitizing
encounter.
The immune system employs many potent effector mechanisms that have the ability to
destroy a broad range of microbial cells and to clear a broad range of both toxic and
allergenic substances. It is critical, therefore, that the immune response is able to avoid
unleashing these destructive mechanisms against the mammalian hosts own tissues. The
ability of the immune response to avoid damaging self-tissues is referred to as self-tolerance.
Because failure of self-tolerance underlies the broad class of autoimmune diseases, this
process has been extensively studied. It is now clear that mechanisms to avoid reaction
against self-antigens are expressed in many parts of both the innate and the adaptive immune
response. The mechanisms that underlie protection of normal self-tissues from immune
damage will be discussed as each of the major effector arms of the host immune response is
introduced.
Because an important aspect of the T cell arm of the immune system is to recognize host
cells that are infected by viruses, intracellular bacteria or other intracellular parasites, T cells
have evolved an elegant mechanism that recognizes foreign antigens together with selfantigens as a molecular complex (see Antigen Recognition by T Lymphocytes below).
This requirement that T cells recognize both self-structures and foreign antigens makes the
need for these cells to maintain self-tolerance particularly important.
Broadly defined, the innate immune system includes all aspects of the hosts immune
defense mechanisms that are encoded in their mature functional forms by the germ-line
genes of the host. These include physical barriers, such as epithelial cell layers that express
tight cell-cell contacts (tight junctions, cadherin-mediated cell interactions, and others), the
secreted mucus layer that overlays the epithelium in the respiratory, gastrointestinal and
genitourinary tracts, and the epithelial cilia that sweep away this mucus layer permitting it to
be constantly refreshed after it has been contaminated with inhaled or ingested particles. The
innate response also includes soluble proteins and bioactive small molecules that are either
constitutively present in biological fluids (such as the complement proteins, defensins, and
ficolins13) or that are released from cells as they are activated (including cytokines that
regulate the function of other cells, chemokines that attract inflammatory leukocytes, lipid
mediators of inflammation, reactive free radical species, and bioactive amines and enzymes
that also contribute to tissue inflammation). Lastly, the innate immune system includes
membrane bound receptors and cytoplasmic proteins that bind molecular patterns expressed
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on the surfaces of invading microbes. Some aspects of the innate host defenses are
constitutively active (such as the mucociliary blanket overlying many epithelia), and others
are activated following interactions of host cells or host proteins with chemical structures
that are characteristic of invading microbes but that are absent from host cells.
Unlike the innate mechanisms of host defense, the adaptive immune system manifests
exquisite specificity for its target antigens. Adaptive responses are based primarily on the
antigen-specific receptors expressed on the surfaces of T- and B-lymphocytes. Unlike the
germ-line-encoded recognition molecules of the innate immune response, the antigenspecific receptors of the adaptive response are encoded by genes that are assembled by
somatic rearrangement of germ-line gene elements to form intact T cell receptor (TCR) and
immunoglobulin (B cell antigen receptor; Ig) genes. The assembly of antigen receptors from
a collection of a few hundred germ-line-encoded gene elements permits the formation of
millions of different antigen receptors, each with potentially unique specificity for a
different antigen. The mechanisms governing the assembly of these B and T cell antigen
receptors and assuring the selection of a properly functioning repertoire of receptor-bearing
cells from the huge randomly generated potential repertoire will be introduced below and
discussed in more detail in chapters 3 and 4.
The innate and adaptive immune systems are often described as contrasting, separate arms
of the host response; however, they usually act together, with the innate response
representing the first line of host defense, and with the adaptive response becoming
prominent after several days, as antigen-specific T and B cells have undergone clonal
expansion. Components of the innate system contribute to activation of the antigen-specific
cells. Additionally, the antigen-specific cells amplify their responses by recruiting innate
effector mechanisms to bring about the complete control of invading microbes. Thus, while
the innate and adaptive immune responses are fundamentally different in their mechanisms
of action, synergy between them is essential for an intact, fully effective immune response.
An intact immune response includes contributions from many subsets of leukocytes. The
different leukocyte subsets can be discriminated morphologically by a combination of
conventional histological stains, and by analysis of the spectrum of glycoprotein
differentiation antigens that are displayed on their cell membranes. These differentiation
antigens are detected by their binding of specific monoclonal antibodies. These cell
phenotype-determining antigens are assigned cluster of differentiation (CD) numbers. There
are currently over 350 defined CD antigens. Updates are issued by Human Cell
Differentiation Molecules (HCDM), an organization that organizes periodic Human
Leukocyte Differentiation Antigen (HLDA) workshops at which newly identified cell
surface molecules are defined and registered. The next HLDA workshop (HLDA9) will be
held in Barcelona, Spain, and the summary of authorized CD molecules will be published at
http://www.hcdm.org/.
Mature, circulating leukocytes differentiate from hematopoietic stem cells (Figure 1). These
stem cells can be recognized by their own spectrum of defining cell surface antigens and can
be purified from bone marrow, peripheral blood, and the placenta.4 The recognition that
pluripotent hematopoietic stem cells can be purified in substantial quantities has accelerated
progress in hematopoietic cell transplantation and provides considerable promise for somatic
cell-based gene therapy. Progress in the field of stem cell therapy is described in chapter 30.
Formation of the full complement of immune system cells begins when a pluripotent
hematopoietic stem cell differentiates into the common myeloid progenitor cell or the
common lymphoid progenitor. The common lymphoid progenitor differentiates further into
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the four major populations of mature lymphocytes: B cells, T cells, natural killer (NK) cells,
and NK-T cells. These lymphocyte subsets can be discriminated by surface phenotype. B
cells are phenotypically defined by their expression of the B cell receptor for antigen,
membrane anchored Ig. Subsets of B cells have been defined that differ in the types of
antigen to which they respond and in the types of antibody they produce. T cells are defined
by their cell surface expression of the TCR, a transmembrane heterodimeric protein that
binds processed antigen displayed by antigen presenting cells (APC). As will be discussed
below, T cells exist in several functionally significant subtypes and subsets of those types.
NK cells are defined morphologically as large granular lymphocytes. They are distinguished
by their lack of either TCR or surface Ig. They recognize their virus-infected or tumor cell
targets using a complex collection of activating and inhibitory cell surface receptors.5 And
NK-T cells share characteristics of both NK cells and T cells.6
Myeloid stem cells (also termed common myeloid progenitors) give rise to the several
different forms of granulocytes, to megakaryocytes and platelets, and to erythrocytes. Cells
of the granulocyte lineage that play prominent immune functions include neutrophils,
monocytes, macrophages, eosinophils, basophils, and mast cells. In some mammals,
platelets also release immunologically significant mediators that expand their repertoire
beyond their role in hemostasis. The immune functions of the classical granulocytes have
been inferred from the immunologically active molecules they produce and from their
accumulation in specific pathological conditions. For example, neutrophils produce large
quantities of reactive oxygen species that are cytotoxic to bacterial pathogens. They also
produce enzymes that appear to participate in tissue remodeling and repair following injury.
Neutrophils accumulate in large quantities at sites of bacterial infection and tissue injury and
possess prominent phagocytic capabilities that permit them to sequester microbes and
particulate antigens internally where they can be destroyed and degraded. Thus, it is clear
that they play a major role in clearance of microbial pathogens and repair of tissue injury.7
More recently, however, neutrophils have been recognized to produce substantial amounts
of the cytokines Tumor Necrosis Factor (TNF) and interleukin (IL)-12 as well as certain
chemokines. This supports an additional immunoregulatory role of neutrophils.
Like neutrophils, monocytes and macrophages are also highly phagocytic for microbes and
particles that have been marked for clearance by binding Ig and/or complement. They
appear to be mobilized shortly after the recruitment of neutrophils and they persist for long
periods at sites of chronic inflammation and infection. In addition to participating in acute
inflammatory responses, they are prominent in granulomatous processes throughout the
body. They use production of nitric oxide as a major mechanism for killing microbial
pathogens, and also produce large amounts of cytokines such as IL-12 and interferon (IFN) giving them a regulatory role in adaptive immune responses. Depending on the nature of
activating signals that are present when macrophages differentiate from immature precursor
cells and when they receive their first activation signal, macrophages can adopt one of
several phenotypes.8 Classically activated macrophages produce large amounts of IFN-,
IL-6, IL-12, and TNF and express potent pro-inflammatory and anti-bacterial activities.
Alternatively activated macrophages are induced by IL-4, IL-10, or IL-13, especially in the
presence of glucocorticoid hormones and express anti-inflammatory functions through their
own production of IL-10, the IL-1 receptor antagonist, and transforming growth factor
(TGF).9 It is likely that further study will identify additional functional macrophage
subsets, establishing additional ways in which these innate immune system cells serve
fundamental immunoregulatory functions.
Eosinophils are readily recognized by their prominent cytoplasmic granules that contain
toxic molecules and enzymes that are particularly active against helminths and other
parasites. The production of eosinophils from the bone marrow and their survival in
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peripheral tissues are enhanced by the cytokine IL-5, making them prominent cells in most
allergic responses.10 Basophils and mast cells are morphologically similar cells that
represent distinct lineages. By virtue of the cell surface expression of high affinity receptors
for IgE (FcRI), they are key initiators of immediate hypersensitivity responses and the host
response to helminthic parasites, releasing histamine and other preformed mediators from
their granules and producing important quantities of lipid mediators that stimulate tissue
inflammation, edema, and smooth muscle contraction. Recent studies have demonstrated
that in addition to their role in immediate hypersensitivity responses, mast cells play
prominent roles in the host response to bacterial infection as well. Importantly, mast cells
and, more prominently, basophils can release substantial amounts of IL-4, suggesting that
they can play important roles in the induction of allergic immune responses.11
Phagocytic cells of the monocyte/macrophage lineage also play key roles in the adaptive
immune response by taking up microbial antigens, processing them by proteolysis to peptide
fragments, and presenting them in forms that can activate T responses. Additional cells in
this lineage include Langerhans cells in the epidermis, Kupffer cells in the liver, and
microglial cells in the central nervous system. The most potent types of APC are the broad
class of dendritic cells that are present in most tissues of the body and concentrated in the
secondary lymphoid tissues.12 All of these cells express both class I and class II major
histocompatibility complex (MHC) molecules that are used to permit recognition of
processed antigen by the TCR on T cells (see below). All MHC bearing cells appear to have
the potential to express APC function if stimulated appropriately. In addition to the
conventional dendritic cells described above, which have been thought to be derived from
myeloid precursor cells (Figure 1), a second type of dendritic cell is recognized. These cells
are designated plasmacytoid dendritic cells because of their histological morphology. They
can produce very high levels of type I interferon and are thought to play special roles in
antiviral host defense and autoimmunity.13 Recent studies of dendritic cell differentiation
indicate that both myeloid stem cells and common lymphoid progenitors can give rise to
both conventional dendritic cells and plasmacytoid dendritic cells, most likely through a
dendritic cell precursor that is defined by its expression of the fms-like tyrosine kinase
receptor-3 (Flt3).14, 15
A major challenge faced by the immune system is to identify host cells that have been
infected by microbes that then use the cell to multiply within the host. Simply recognizing
and neutralizing the microbe in its extracellular form does not effectively contain this type
of infection. The infected cell that serves as a factory for production of progeny microbes
must be identified and destroyed. In fact, if the immune system were equally able to
recognize extracellular microbes and microbially infected cells, a microbe that managed to
generate large amounts of extracellular organisms or antigen might overwhelm the
recognition capacity of the immune system, allowing the infected cells to avoid immune
recognition. A major role of the T cell arm of the immune response is to identify and destroy
infected cells. T cells can also recognize peptide fragments of antigens that have been taken
up by APC through the process of phagocytosis or pinocytosis. The way the immune system
has evolved to permit T cells to recognize infected host cells is to require that the T cell
recognize both a self-component and a microbial structure. The elegant solution to the
problem of recognizing both a self-structure and a microbial determinant is the family of
MHC molecules. MHC molecules (also called the human leukocyte-associated [HLA]
antigens) are cell surface glycoproteins that bind peptide fragments of proteins that either
have been synthesized within the cell (class I MHC molecules) or that have been ingested by
the cell and proteolytically processed (class II MHC molecules).
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There are three major HLA class I molecules, designated HLA-A, -B, and -C, each encoded
by a distinct gene. The class I HLA molecules are cell surface heterodimers consisting of a
polymorphic transmembrane 44-kd -chain (also designated the class I heavy chain)
associated with the 12-kd non-polymorphic 2-microglobulin (2m) protein.16 The -chain
determines whether the class I molecule is an HLA-A, -B, or C molecule. The HLA-A, -B,
and -C -chain genes are encoded within the MHC on chromosome 6 (Figure 2), and the 2microglobulin gene is encoded on chromosome 15. The -chain gene encodes three
extracellular domains (designated 1, 2, and 3), a transmembrane domain and a short
intracellular domain that anchors the protein in the cell membrane. The 3 domain consists
of 5 antiparallel -strands that form an immunoglobulin-type fold (Figure 3). The 1 and 2
domains each encode an -helix and several -strands. The 1 and 2 domains associate with
each other with their -strands forming a platform on which the two -helices rest. This
forms a groove in which antigenic peptides can bind. This complex of class I MHC
molecule and antigenic peptide produces a composite structure that is the molecular target of
the TCR. The TCR contacts both the antigenic peptide and the flanking -helices. The TCR
has no measurable affinity for the antigenic peptide alone, and very low affinity for MHC
molecules containing other peptides. These observations form the molecular basis for the
phenomenon of MHC restriction described by studies of Zinkernagel and Doherty, in
which they recognized that T cells could only recognize their specific antigen when it was
presented in association with a specific self-MHC molecule.17
A key biological consequence of requiring the T cell to recognize antigenic peptides only
when they are bound in the groove of an HLA molecule is that this permits the T cell to
ignore free extracellular antigen, and to focus rather on cells that contain the antigen. In the
case of cells that are infected by a pathogenic microbe, this permits the T cells to focus their
response on the infected cells. The 3 domain of the class I heavy chain interacts with the
CD8 molecule on cytolytic T cells. This restricts recognition of antigenic peptides that are
presented in class I HLA molecules to CD8+ cytolytic T cells. The binding of CD8
expressed by the T cell to the 3 domain of the class I molecule expressed by the APC
strengthens the interaction of the T cell with the APC and helps assure that full activation of
the T cell occurs.18
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Peptide fragments are generated from cellular proteins by the action of the proteasome, a
proteolytic factory composed of over 25 subunits.19 Proteasomes are expressed
constitutively in all cell types where they function in cellular homeostasis. Stimulation of
cells with IFN- activates them for the production of antigenic peptide fragments that can be
presented in HLA class I molecules. This activation induces the production of a variant of
the proteasome termed the immunoproteasome. Two of the subunits of the constitutively
expressed proteasome are replaced in the immunoproteasome by the IFN- induced LMP2
and LMP7 proteins, both of which are encoded within the HLA complex in the interval
between the HLA-DP and the HLA-DQ gene loci (Figure 2). The LMP2 and LMP7 proteins
alter the proteolytic specificity of the proteasome, enhancing the production of peptide
fragments of appropriate length and charge for binding in the groove of the HLA class I
proteins. The addition of another IFN- induced protein termed the PA28 proteasome
activator also enhances the generation of antigenic peptides that are favorable for
presentation in HLA class I molecules.20 After exiting from the immunoproteasome, peptide
fragments are transported into the endoplasmic reticulum (ER) by the action of a specific
multi-subunit transmembrane transporter. This transporter contains two ATP-binding
cassette subunits designated TAP-1 and TAP-2 (Transporters Associated with antigen
Presentation) encoded by genes that are located within the MHC gene complex in the same
region that encodes LMP2 and LMP7 (Figure 2). Once in the ER, the peptides are loaded
into the class I protein binding groove under the direction of the ER protein tapasin with the
help of the calcium-binding chaperone protein calreticulin and the oxidoreductase Erp57.21,
22 Prior to its interaction with -microglobulin, the class I protein is maintained in a
2
conformation that favors interaction with peptide fragments by association with the
chaperone protein calnexin. Interaction with 2-microglobulin stabilizes the complex,
causing dissociation of calnexin, and permitting transport of the peptide-loaded class I
molecule via the Golgi complex into exocytic vesicles that release the intact complexes onto
the cell surface. This pathway is well-adapted to delivering viral peptides produced in a
virus infected cell to the cell surface bound to class I HLA molecules in a form that can be
recognized by cytotoxic CD8+ T cells. It may also be used to present tumor specific protein
fragments that may be useful targets for anti-tumor immunotherapy.
Studies over the past several years have shown that under certain circumstances exogenous
antigens (synthesized outside of the APC) can also be internalized by endocytosis and
presented in HLA class I molecules. This uptake of exogenous antigens and display to T
cells in HLA class I proteins is known as cross presentation.23 Cross presentation is
particularly important in antiviral immunity where it helps the host to overcome the ability
of some viruses to suppress antigen processing through the endogenous pathway.24
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region encodes 1 polymorphic chain (16 alleles) and 1 polymorphic chain (118 alleles).
Because both the chains and the chains of the HLA-DQ and HLA-DP proteins are
polymorphic, each person can express 4 different HLA-DQ and 4 different HLA-DP
proteins based on pairing between the gene products of both the maternal and the paternal
chromosome. Furthermore, because the minimally polymorphic HLA-DR chain can pair
with an HLA-DRB1 and an HLA-DRB3 chain from both the maternal and the paternal
chromosome, each person can express 4 distinct HLA-DR proteins as well. Each of these
has the potential to bind a large repertoire of antigenic peptides, making it difficult for a
pathogenic microbe to mutate its structure to a form that cannot be recognized by binding in
an HLA class II protein.
Each chain of the class II proteins contains a short cytoplasmic anchor, a transmembrane
domain, and two extracellular domains designated for the chain 1 and 2, and for the
chain 1 and 2.16 When the and chains pair, the 1 and 1 domains combine to form a
peptide-binding groove very similar in structure to that formed by the association of the 1
and 2 domains of the class I proteins. The 2 and 2 domains of the proteins provide a
support for this peptide-binding domain and the 2 domain also interacts with the CD4
molecule. This provides a mechanism by which CD4 expressed on helper T cells can
enhance the interaction between these T cells and the class II-expressing APC in a fashion
similar to the way binding of the HLA class I molecule by CD8 enhances cytotoxic T cell
activation.25
The class II proteins are expressed constitutively on B cells, dendritic cells, monocytes and
macrophages, all cells that present antigens to CD4+ T cells. Expression of MHC class II
proteins can also be induced on many additional cell types, including epithelial and
endothelial cells following stimulation with IFN, permitting these cells to present antigens
to CD4+ T cells at sites of inflammation.
Antigens that are presented by class II proteins are loaded into the class II peptide-binding
groove via the exogenous pathway that starts by endocytosis or phagocytosis of
extracellular proteins (Figure 5). The exogenous antigens include antigenic proteins of
extracellular pathogens such as most bacteria, parasites, and virus particles that have been
released from infected cells and taken up by phagocytosis as well as environmental proteins
and glycoproteins such as pollens and venoms, and alloantigens. The ingested antigens are
processed to linear peptide fragments by proteolysis after fusion of lysosomes with the
phagocytic vacuoles or endosomes to form an acidic compartment.26 The peptide fragments
then accumulate in the MHC II loading compartment where they encounter nascent class II
proteins. The and chains of the class II molecules are synthesized in the ER. In order to
protect the class II molecules peptide-binding groove so that it can later accommodate an
antigenic peptide, the and chains associate with the non-polymorphic invariant chain (Ii),
assisted by the chaperone protein calnexin. A portion of the Ii chain designated CLIP (class
II-associated invariant-chain peptide) lies in the peptide-binding groove of the class II
heterodimer, preventing binding of antigenic peptides. Once the class II-Ii complex has
formed, it dissociates from calnexin and is transported to the class II loading compartment.27
In the class II loading compartment, the bulk of the invariant chain is degraded by acid
proteases such as cathepsins and exchange of the CLIP peptide for an antigenic peptide is
catalyzed by the action of the HLA-DM molecule, resulting in the formation of a mature
class II protein.28 The class II proteins loaded with antigenic peptide are then delivered to
the cell surface by fusion of the class II+ endosome to the plasma membrane.
Association of HLA Types and Disease Susceptibility
Epidemiological studies have demonstrated that over 40 diseases are found more frequently
in individuals carrying certain HLA class I or II alleles than in the general population.29 The
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magnitude of these effects can be quite large, but are probably never absolute. For example,
they range from the finding that between 90 and 95% of Caucasian patients with ankylosing
spondylitis are HLA-B2730 to the observation that between 30% and 50% of Caucasian
patients with type I diabetes mellitus are heterozygous for HLA-DQ2/DQ8.31 Interestingly,
HLA-DQ6 appears to provide dominant protection from development of type I diabetes.
Most diseases that show linkage of susceptibility to particular HLA genes have a prominent
autoimmune character. Although the mechanisms by which HLA genotypes control
susceptibility to these diseases remains imprecisely defined, it is likely that the participation
of HLA molecules in the establishment of immune tolerance or permitting immune
recognition of environmental antigens underlies this phenomenon.32, 33 Protective HLA
gene alleles may mediate the elimination in the thymus of potentially pathogenic T cells,
whereas susceptibility HLA gene alleles may fail to contribute appropriately to elimination
of pathogenic T cells. HLA genotypes can also underlie responsiveness or nonresponsiveness to certain vaccines. For example, subjects who are HLA-DR3 have a
substantially increased incidence of non-responsiveness to vaccination with hepatitis B
surface antigen34 and subjects who are HLA-DRB1*03 or HLA-DQA1*0201 have an
increased incidence of seronegativity after measles vaccination.35
HLA-independent Presentation of Antigen
Antigen presentation by class I and class II HLA molecules to CD8+ and CD4+ T
lymphocytes is limited to protein antigens. Initially, it was thought that responses to
polysaccharide antigens and lipid antigens was restricted to T cell-independent responses
that resulted in direct activation of B cells by an antigen with a repeating structure; however,
recently it has become clear that there is a class of T cells that recognizes antigens presented
by molecules that are not classical HLA class I or class II antigens. One of these classes of T
cells uses an antigen receptor composed of and chains and recognizes lipid antigens that
are presented bound to CD1 molecules.6 CD1 molecules are structurally related to class I
HLA molecules, being transmembrane proteins with 3 extracellular domains and associating
with 2-microglobulin. There are 5 human CD1 isoforms designated CD1a-CD1e, encoded
by linked genes that are not associated with the MHC. X-ray crystallography shows that the
1 and 2 domains of CD1 molecules associate like class I MHC molecules to form a
binding groove that can accommodate glycolipid components of microbial pathogens.36
CD1-glycolipid complexes can also serve as targets for recognition by T cells that use the
TCR (see below). This presentation of microbial glycolipids by CD1 molecules appears to
underlie the MHC-independent recognition of mycobacteria by both and T cells.
Glycosphingolipids, a class of carbohydrate-containing lipids that are found in both
eukaryotic and prokaryotic cells can also be presented by the CD1d molecule to NK-T cells,
leading to their release of large quantities of immunoregulatory cytokines.37 Human T
cells can also recognize target cells by virtue of their expression of the stress-inducible
MHC class I-related chains A and B (MICA and MICB). MICA and MICB are encoded by
genes that lie between the TNF gene cluster in the class III region of the MHC and the HLAB locus in the class I region (Figure 2). They share structural characteristics with the class I
protein heavy chains but appear not to associate with 2microglobulin and not to bind
antigenic peptides. Rather, they act as stress-induced molecules that are targets for intestinal
T cells, further expanding the repertoire of molecules that can contribute to activation of
responding T lymphocytes. In addition to the two functional MICA and MICB genes, there
are at least three inactive MIC pseudogenes encoded within the class I region of the MHC
(Figure 2).38
T Lymphocytes
The major class of T cells is defined by its surface expression of the TCR. This receptor
has evolved primarily to recognize peptide antigens presented in a complex with class I or
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class II MHC proteins. -T cells differentiate into several different subsets, some of which
(CD8+ T cells) act primarily to kill cells infected with intracellular microbes, and others
(CD4+ T cells) act primarily to regulate the cellular and humoral immune responses. A small
subset of -T cells which expresses the NK1.1 (CD161) NK cell antigen (NK-T cells) are
usually CD4 and CD8 double negative, recognize glycolipid antigens presented by the CD1d
molecule, and appear to be immunoregulatory based on their ability to release rapidly large
quantities of the cytokines IFN-, IL-4, granulocyte-macrophage colony stimulating factor
(GM-CSF), TNF, and others.39 Details of the mechanisms by which T cells develop,
acquiring their antigen specificity, and then are regulated as they encounter antigen in the
peripheral tissues are discussed in Chapter 3. An introductory overview is presented here.
T Cell Development
Each individual T cell bears antigen receptors of a single specificity. A repertoire of T cells
that can protect against the vast universe of microbial pathogens must, therefore, include a
very large number of cells encoding a huge array of discrete TCR. These receptors are
somatically assembled from variable, diversity, and joining gene elements to generate
mature VJ chains and VDJ chains (see chapter 3). The assembly of these gene elements
is initiated by the lymphoid-specific RAG1 and RAG2 proteins which cleave the DNA near
the V, D, and J segments and the gene segments are rejoined by a collection of nonlymphoid-specific DNA repair enzymes including DNA-dependent protein kinase (DNAPK), Ku, XRCC4, XLF, DNA ligase IV, and the Artemis nuclease.40 XRCC4, XLF, and
DNA-PK help recruit the enzyme, terminal deoxynucleotidyl transferase (TdT), which adds
deoxynucleotides into some of the VDJ junctions providing extra junctional diversity to the
recombined gene sequences.41 The action of these recombinase enzymes results in the V, D,
and J gene elements assembling in an apparently random process, producing huge diversity
of receptor sequences, but also frequently producing non-functional genes. Selection of cells
carrying functional TCR genes occurs in the thymus (Figure 6), a complex lymphoid organ
located in the anterior mediastinum at the base of the neck.42 The thymus contains 3
compartments. The first, the subcapsular zone, is where bone marrow-derived prothymocytes begin to differentiate, proliferate, and rearrange their TCR chains. The cells
then move to the thymic cortex where the chain gene elements rearrange, potentially
forming a functional, mature TCR. In the cortex, cells test whether their receptors have
sufficient affinity for self-MHC molecules to permit them ultimately to recognize antigenMHC complexes. This involves interactions between the developing lymphocyte and the
specialized cortical epithelium.43 If the lymphocyte fails this positive selection, then it
undergoes apoptosis and is cleared by thymic cortical macrophages. Finally, in the thymic
medulla, cells are screened for potential autoreactivity. This screening includes testing for
reactivity for an extensive array of tissue-specific proteins that are expressed by a population
of thymic medullary epithelial cells under the control of a gene called AIRE (autoimmune
regulator). Defective expression of AIRE gives rise to the severe autoimmune syndrome
called autoimmune polyendocrinopathy-candidiasis-ectodermal dystrophy (APECED).44
Cells that recognize self-peptides expressed by these epithelial cells are removed by
apoptosis, and cells that have survived this negative selection are exported to the circulation.
Fewer than 5% of the developing T cells survive positive and negative selection.
Approximately 9095% of circulating T cells use the TCR described above. The other 5
10% use an alternate heterodimeric TCR composed of and chains. The and chains also
assemble by RAG1/RAG2-mediated rearrangement of V, D (for the chain only), and J
elements. A portion of the T cells is generated in the thymus, but a major fraction appears
to be generated in an extrathymic compartment, resulting in cells that largely populate the
GI tract.45
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The antigen-specific and chains of the TCR associate with invariant accessory chains
that serve to transduce signals when the TCR binds to antigen-MHC complexes.46 These
accessory chains make up the CD3 complex, consisting of the transmembrane CD3, CD3,
and CD3 chains plus a largely intracytoplasmic homodimer of two CD3 chains. Although
the stoichiometry of the CD3 complex is not definitively established, it appears that each
TCR pair associates with a CD3 heterodimer, a CD3 heterodimer, and a CD3
homodimer (Figure 7).
Interaction of the TCR/CD3 complex with antigenic peptide presented in an HLA molecule
provides only a partial signal for cell activation. Full activation requires the additional
participation of a co-stimulatory molecule, such as CD28 on the T cell and CD80 (also
designated B7.1) or CD86 (B7.2) on the antigen-presenting cell (Figure 7).47 In fact,
interaction of peptide-MHC with the TCR without a co-stimulator can lead to an anergic
state of prolonged T cell non-responsiveness.
The cytoplasmic portions of each of the CD3 chains contain sequence motifs designated
immunoreceptor tyrosine-based activation motifs (ITAM). When key tyrosines in these
ITAMs are phosphorylated by the receptor-associated kinases Lck and Fyn, this initiates an
activation cascade involving the proteins ZAP-70, and farther downstream LAT, and
SLP-76. Activation of these proteins leads to stimulation of phospholipase C, activation of
the G proteins Ras and Rac, and both protein kinase C and the mitogen-associated protein
(MAP) kinases. Together, this complex of activation events leads to activation of genes that
control lymphocyte proliferation and differentiation.
The pathways that down regulate this activation pathway are becoming increasingly well
defined. The membrane molecule CD45 is a key tyrosine phosphatase that occupies a central
position in this de-activating process. In addition, a specific receptor-ligand pair, PD-1
(programmed death-1) and PD-L1 (programmed death ligand 1), transduces signals to the
activated lymphocyte to inhibit its proliferation and effector functions, thus extinguishing
the T cell response.48 Mutations affecting the function of many of the molecules involved in
intracellular lymphoid cell signal transduction processes underlie congenital primary
immunodeficiency syndromes (chapter 15).
T Cell Subpopulations
During their progress through the thymus, T cells differentiate into discrete
subpopulations, each with defined repertoires of effector functions. The major subsets are
defined by their selective surface expression of CD4 or CD8. In the thymus, most
developing T cells follow a developmental program in which in the cortex they first express
neither CD4 nor CD8 (double negative) and then express both CD4 and CD8 (double
positive [DP]).49 DP cells are tested by positive selection in the thymic cortex and those that
are selected on class I MHC molecules become CD4CD8+, and those that are selected on
class II MHC molecules become CD4+CD8. The fact that the CD4 molecule contributes to
a stable interaction of the developing T cell with class II MHC molecules on the selecting
APC and that CD8 contributes to interactions with class I molecules is central to the
association of CD4 with class II MHC restricted antigen recognition and of CD8 with class I
restricted antigen recognition. Cells that survive positive selection then move to the thymic
medulla for negative selection and export to the periphery. In the blood and secondary
lymphoid organs, 6070% of T cells are CD4+CD8 (CD4+) and 3040% are CD4CD8+
(CD8+). CD4+ T cells are generally designated helper cells and activate both humoral
immune responses (B cell help) and cellular responses (delayed type hypersensitivity
responses, others). CD8+ cells show a major cytotoxic activity against cells infected with
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intracellular microbes and against tumor cells, but also contain regulatory cells that downregulate immune responses (suppressor cells). A portion of the circulating CD4+ T cells play
an important regulatory role that acts to down modulate immune responses. These regulatory
T (Treg) cells fall into two groups. The first group develops its regulatory function in the
thymus and is known as natural Treg cells. These cells are characterized by surface
expression of the CD4 and CD25 antigens and by nuclear expression of the forkhead box P3
transcription factor (Foxp3) that is essential for their development. A major portion of this
populations regulatory activity is due to its secretion of the immunomodulatory cytokines
TGF and IL-10.50 Under some conditions, suppression of effector T cell proliferation by
Treg cells requires cell-cell contact. In this situation, it has been reported that TGF acts in a
membrane-associated form.51 The second group of Treg cells is thought to differentiate in
the periphery from nave CD4+ T cells. Because they appear to develop in response to
stimulation with specific antigen, they are called adaptive or induced Treg cells. Their
differentiation appears to depend on the presence of IL-10 during their initial activation.
Expression of Foxp3 is variable in this subset, and IL-10 is a prominent secreted product
with TGF also participating.52 The phenotype of these cells can be unstable, with Foxp3
expression disappearing soon after withdrawal of the inductive IL-10 or TGF. Recent
studies have indicated that epigenetic modification of the Foxp3 locus, in the form of both
histone acetylation and altered DNA methylation in the area around the Foxp3 promoter, are
essential for establishment of stable expression of Foxp3 and maintenance of the Treg
phenotype.53
Approximately 510% of T cells in the peripheral blood, lymph nodes, and spleen are
CD4CD8. Some of these cells use TCR and others use TCR. Double negative cells
do not recognize antigen in the context of MHC class I or class II. Some of these cells
recognize antigen in the class I-related protein CD1 that is adapted to presentation of
glycolipid components of mycobacteria and other microbes.36 A subset of double negative
T cells recognizes the MHC class I chain-related proteins designated MIC.38
Both CD4+ and CD8+ T cells differentiate into functionally distinct subsets following
exposure to antigen. This is best described for the transition of CD4+ T cells from nave to
effector populations. Resting nave CD4+ T cells (designated T helper cells, Th) release very
low levels of cytokines. Early after stimulation by antigen and APC, the Th cells begin to
produce IL-2 and are designated Th0. As the Th cells continue to respond to the activating
signal, they progress towards polar extremes of differentiation designated Th1, Th2, and
Th17 depending on the nature of the cytokines present at the site of activation.54 IL-12
produced by macrophages or NK cells induces differentiation towards Th1, IL-4 produced
by NK1.1+ T cells, basophils, or mast cells induces differentiation towards Th2 and TGF
and IL-6 produced by yet to be defined cells induce differentiation towards Th17. Th1 cells
are characterized by their expression of the transcription factor t-bet and by the production
of IL-2, IFN-, and lymphotoxin. Th2 cells are characterized by their expression of the
transcription factor GATA-3 and produce IL-4, IL-5, IL-9, IL-13, and GM-CSF, and Th17
cells express the transcription factor RORC2 and produce the cytokines IL-6 and IL-1755
(see chapter 3). Th17 cells are induced early in the adaptive response to extracellular
bacteria and help to recruit the neutrophil response that eliminates these pathogens. They
also direct the destructive inflammatory responses that are part of many autoimmune
diseases. Th1 and Th2 cells often participate together in immune responses; however, after
prolonged immunization, the response can become dominantly Th1-like or Th2-like.
Generally, Th1 cells support cell mediated immune responses, and Th2 cells support
humoral and allergic responses. CD8+ T cells also can manifest type 1 and type 2 cytokine
responses, in which case the cells are designated T cytotoxic cell type 1 (Tc1) and T
cytotoxic cell type 2 (Tc2).56 Understanding the factors that govern whether a Th response
adopts a predominantly Th1-type, a Th2-type, or a Th17-type response is crucial to the
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B Lymphocytes
B Cell Development and the B Cell Antigen Receptor
B cells constitute approximately 15% of peripheral blood leukocytes. They are defined by
their production of Ig. Except as noted below, Ig molecules are composed of two identical
50 kDa heavy chains and two identical 25 kDa or light chains (see chapter 3). The amino
terminal portions of the heavy and light chains vary in amino acid sequence from one
antibody molecule to another. These variable portions are designated VH and V or V,
respectively. The juxtaposition of one VH segment and one V or V segment creates the
antigen-binding portion of the intact Ig molecule. The variable regions of both the heavy and
light chains contain three sub-regions that are highly variable between different antibody
molecules. These hypervariable sequences are brought together in the Ig protein to form the
antigen-binding domain of the molecule. Thus, each Ig has two identical antigen binding
sites. The carboxyl terminal portions of the heavy and light chains are constant in each
subclass of antibody. The heavy chain constant regions pair to form the Fc domain of the
molecule that is responsible for most of the effector functions of the Ig molecule, including
binding to Fc receptors and activating the complement system.
The genes encoding the light chain are encoded on chromosome 2, and the genes encoding
the light chain are on chromosome 22. The complex heavy chain locus is encoded on
chromosome 14. The light chain and heavy chain loci are each composed of a series of V
(variable) gene elements, followed by several D (diversity) segments (for the heavy chain
gene only), some J (joining) segments, and C (constant region) exons. The constant regions
of both the and the light chain genes are encoded as single exons. The heavy chain gene,
in contrast, contains exons that encode 9 different constant regions that are used to produce
the different classes and subclasses of Ig (Table 1).
B cells differentiate from hematopoietic stem cells in the bone marrow. It is here that their
antigen receptors (surface Ig) are assembled from genetic building blocks in a RAG1/
RAG2-mediated process similar to that used for the production of functional TCR.59 The
amino terminal portion of each heavy chain is created by somatic joining of genes encoding
a variable (VH), diversity (DH), and joining (JH) region. Joining of genes encoding variable
and constant light chain gene elements generates the amino terminal portion of the light
chain. The VDJ junctions formed by this recombination make up the 3rd hypervariable
region that contributes to the antigen-binding site. The amino acid sequence diversity of the
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encoded sequences added into the junction sites by the action of the enzyme TdT that is
expressed in developing B cells during the time this gene rearrangement is occurring.
Differentiation of stem cells to the B lineage depends on bone marrow stromal cells that
produce IL-7. The developing B cells follow a program of differential surface antigen
expression and sequential heavy and light chain gene rearrangement (Figure 8). First, the
recombinase enzyme complex catalyzes the fusion of one of the DH region genes to a JH
region gene with the deletion of the intervening DNA sequences. This DHJH recombination
occurs on both chromosomes. Next, the recombinase joins one of the VH region genes to the
rearranged DHJJ gene. TdT is expressed during this period, resulting in the addition of
random nucleotides into the sites of DH-J and VH-DHJH joining, adding to the potential
diversity of amino acid sequences encoded by the rearranged VHDHJH gene. The rearranged
VHDHJH element forms the most 5 exon of this rearranged heavy chain gene, and is
followed downstream by exons encoding the constant region of the m chain that pairs with a
light chain to produce IgM and farther downstream by exons encoding the constant region of
the d chain that is used to make IgD. chains and chains are produced as a result of
alternative RNA splicing of the VHDHJH exon to either the exons or the exons. If the
rearrangements of the VH, DH, and JH elements yields a heavy chain transcript that is inframe and encodes a functional heavy chain proteins, this heavy chain is synthesized and
pairs in the cell with two proteins, 5 and VpreB, which act as a surrogate light chain
(Figure 8). Expression of this pre-B cell receptor on the cell surface prevents VH to DHJH
rearrangement on the other chromosome, assuring that the developing B cell produces only
one antigenic specificity. This process is called allelic exclusion. If the first VHDHJH
rearrangement is out of frame and does not produce a functional heavy chain protein, then a
VH gene proceeds to rearrange on the other chromosome in a second attempt to generate a
successful heavy chain rearrangement. If this second rearrangement is unsuccessful, the cell
undergoes apoptosis and is removed.
Once a functional heavy chain is produced, the cell down regulates its TdT gene and
initiates light chain rearrangement. First, a V element rearranges to a J element. If this
forms a functional light chain, then the light chain pairs with the heavy chain to form a
functional Ig protein and further light chain rearrangement stops. If the first rearrangement
fails, then rearrangement proceeds on the other chromosome. If that fails, then
rearrangement of the chains proceeds. The RAG1 and RAG2 genes are only expressed
during times of heavy and light chain rearrangement, except that some B cells that express
autoreactive receptors appear able to re-express their RAG genes and undergo receptor
editing by secondary rearrangements of their already rearranged Ig genes.60 These
processes result in the assembly of the antigen-binding component of the B cell receptor.
Like the TCR, the fully mature B cell receptor also includes additional transmembrane
proteins designated Ig and Ig that activate intracellular signals after receptor binding to
antigen.61, 62 B cells also have a co-receptor complex consisting of CD19, CD81, and CD21
(complement receptor 2) that is activated by binding to the activated complement protein
C3d.63 Both Ig and Ig have ITAM domains in their cytoplasmic regions, and utilize
similar signal transduction pathways compared to that for T cells. The B cell pathway
includes the src-family of kinases Blk, Fyn, and Lyn that phosphorylate the ITAMs on the
Ig and Ig chains. The activation signal is then passed via the tyrosine kinase Syk and the
linker protein BLNK to the downstream signaling components phospholipase C and guanine
nucleotide exchange factors. Ultimately, as in T cells, activation of protein kinase C,
calcium mobilization, and Ras/Rac-dependent activation of MAP kinases leads to activation
of new gene transcription that causes cell proliferation and maturation.
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Nave B cells express on their cell surfaces IgM and IgD. These two Ig isotypes are
expressed by alternative splicing of the same VHDHJH exon to the m and d heavy chain
exons. For all heavy chain genes, alternative splicing also permits expression of both
membrane-bound (splicing in a transmembrane exon) and secreted (transmembrane exon
spliced out) antibody. As B cells mature under the influence of helper T cells, T cell-derived
cytokines induce isotype switching. Isotype switching is a process of DNA rearrangement
mediated in part by the RNA-editing enzyme activation-induced cytidine deaminase (AID),
uracil-DNA glycosylase (UNG), the endonuclease APE1, and the DNA repair enzyme
DNA-PK. Switching moves the rearranged VHDHJH exon into a position immediately
upstream of alternative heavy chain exons. This permits a functionally rearranged VHDHJH
exon to be used to produce antibodies of different isotypes but the same antigenic
specificity.64 T cell derived IL-10 causes switching to IgG1 and IgG3. IL-4 and IL-13 cause
switching to IgE, and TGF causes switching to IgA. IFN- or some other undefined
product of Th1 cells appears to induce switching to IgG2.
At the same time as B cells undergo isotype switching, an active process produces
mutations, apparently randomly, in the antigen-binding portions of the heavy and light
chains. This process, designated somatic mutation, also appears to require AID, UNG,
APE1, and DNA repair enzymes.65 If these mutations result in loss of affinity for the
antigen, the cell loses important receptor-mediated growth signals and dies. If, however, the
mutations resulted in increased affinity for the antigen, then the cell producing that antibody
has a proliferative advantage in response to antigen and grows to dominate the pool of
responding cells. Somatic mutation and clonal expansion of mutated cells occurs in the
germinal centers of secondary lymphoid tissues.66
T Cell-Dependent B Cell Responses
Antigens that activate T cells as well as B cells establish Ig responses in which T cells
provide help for the B cells to mature. This maturation includes both induction of isotype
switching, in which the T cell cytokines control the isotype of Ig produced, and activation of
somatic mutation. The cellular interactions underlying T cell help are driven by the specific
antigen and take advantage of the ability of B cells to serve as APC. B cells that capture
their cognate antigen via their membrane Ig can internalize the antigen and process it
intracellularly for presentation on the cell surface in the B cells class II HLA proteins.
Uptake of antigen induces increased class II expression and expression of CD80 and CD86.
T cells activated by this combination of co-stimulator and antigen-class II complex on the B
cell then signal reciprocally to the B cell by the interaction of the T cell CD40 ligand
(CD40L) with B cell CD40. Signaling through CD40 is essential for induction of isotype
switching, and human patients with defects in the X chromosome encoded CD40L gene
manifest X-linked hyper-IgM syndrome and patients with mutant CD40 show autosomal
recessive hyper-IgM syndrome.67
Isotype switching and somatic mutations are strongly associated with the development of B
cell memory. Memory responses, defined as rapid induction of high levels of high affinity
antibody after secondary antigen challenge, are characterized by production of IgG, IgA, and
IgE antibodies, and by somatic mutations in the antigen-binding domains of the heavy and
light chains of these antibodies.68 The development of B cell memory is critical to the
success of vaccination against pathogens and also perpetuates the pathology of many
autoimmune and allergic syndromes. Understanding how to enhance or reduce memory
responses will provide important new therapeutic opportunities to the clinical immunologist.
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B cells can also be activated successfully without T cell help. T cell independent B cell
activation occurs without the assistance of T cell co-stimulatory proteins. In the absence of
co-stimulators, monomeric antigens are unable to activate B cells. Polymeric antigens with a
repeating structure, in contrast, are able to activate B cells, probably because they can crosslink and cluster Ig molecules on the B cell surface. T cell independent antigens include
bacterial lipopolysaccharide (LPS), certain other polymeric polysaccharides, and certain
polymeric proteins. Somatic mutation does not occur in most T cell independent antibody
responses. Consequently, immune memory to T cell independent antigens is generally weak.
This is why it is difficult to create fully protective vaccines directed against polysaccharide
components of microbes. Covalent attachment of the polysaccharide component to a carrier
protein, in order to recruit T cell help to the response, can induce a beneficial memory
response. The value of coupling a polysaccharide antigen to a carrier protein was observed
in the Haemophilus influenzae type B vaccine. The original polysaccharide vaccine provided
low antibody titers, and no protection for children less than 18 months of age. The current
conjugate vaccine generally provides protection beginning at 24 months of age.
Lymphoid Tissues
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Cellular interactions are essential for a normally regulated, protective immune response. In
particular, T cell help is needed to generate high affinity antibody with memory against most
protein antigens. A major challenge for the immune system of a nave subject is to bring rare
antigen-specific B cells together with rare antigen-specific T cells and antigen-charged APC.
The primary role of the secondary lymphoid tissues is to facilitate these interactions.
Generally, the secondary lymphoid organs contain zones enriched for B cells (follicles) and
other zones enriched for T cells.69 The B cell zones contain clusters of follicular dendritic
cells (FDC) that bind antigen-antibody complexes and provide sites adapted to efficient B
cell maturation, somatic mutation and selection of high affinity B cells. The T cell zones
contain large numbers of dendritic cells that are potent APC for T cell activation. The tissues
also contain specialized vascular structures for recruitment of cells into the tissue. High
endothelial venules in lymph nodes, Peyers patches, and mucosal associated lymphoid
tissues are vascular sites that efficiently extract nave T and B cells from the circulation into
the lymphoid organ. The marginal sinus probably serves a similar function in the spleen.
Afferent lymphatic vessels provide efficient entry of antigen-charged antigen-transporting
cells (such as epidermal Langerhans cells) from peripheral tissues into lymph nodes.
Efferent lymphatic vessels permit efficient export of antigen-experienced cells back into the
circulation. Programmed release of distinct chemokines within the lymphoid tissues
orchestrate the coming together of antigen-responsive B cells and T cells and then migration
of the activated B cells and selected T cells to the FDC clusters where they can form a
germinal center.70 In addition to chemokines signals that control leukocyte entry into and
migration within secondary lymphoid tissues, it is now understood that specific signals,
especially provided by the lysophospholipid sphingosine 1-phosphate, regulate the egress of
cells out of the lymphoid tissues and into the circulation.71
Although potent adjuvants can induce some degree of affinity maturation in the setting of
congenital absence of lymph nodes and Peyers patches, these secondary lymphoid organs
are generally essential for the induction of an efficient, protective immune response. Ectopic
lymph node-like structure designated tertiary lymphoid tissues can form at sites of chronic
inflammation such as the synovial membrane of a joint affected by rheumatoid arthritis.
Immune reactions ongoing in these tertiary lymphoid tissues can contribute importantly to
the pathogenesis of the inflammatory disease.
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Signaling by Cytokines
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Cytokines act on cells via transmembrane cell surface receptors. Binding of the cytokine to
the receptor elicits its cellular response by activating an intracellular signal transduction
pathway that ultimately leads to induction of new gene transcription and synthesis of new
cellular proteins. Most cytokine receptors signal using one of the Janus kinase (Jak) family
of molecules that then acts on the signal transducers and activators of transcription (STAT)
family of proteins. Specific Jak proteins associate with the cytoplasmic domains of cytokine
receptor. When the receptor is activated by binding the cytokine, the Jak phosphorylates its
respective STAT protein, causing the STAT to dimerize, and translocate into the nucleus
where it then initiates new gene transcription. The essential role of Jak and STAT proteins in
immune regulation is seen in individuals with inherited deficiency of these molecules (see
chapter 12). Jak3 interacts with the c protein, a subunit of several cytokine receptors
including the receptors for IL-2, IL-4, IL-7, IL-9, IL-15 and IL-21. Deficiency of the
autosomally encoded Jak3 protein causes autosomal recessive severe combined immune
deficiency (SCID).72 Deficiency of the X chromosome encoded c protein causes X-linked
SCID.73 Mutation of STAT1 causes susceptibility to infection with mycobacteria and a
variable increase in susceptibility to virus infections because of impaired ability to respond
to signals from either type I or type II interferons.74 Homozygous deficiency of STAT3 in
mice is embryonic lethal, but heterozygous deficiency of STAT3 in humans causes
autosomal dominant hyper-IgE syndrome associated with deficiency of Th17 cell
differentiation.75 Deficiency of STAT4 blocks IL-12 signal transduction resulting in
impaired development of Th1 cells. And STAT6 deficient mice showed impaired signaling
through the IL-4 receptor and inability to generate Th2 cell-dependent responses.76
While the adaptive T and B cell immune responses provide important protection for the host
and permit the development of immune memory, mutations in elements of the innate
immune response demonstrate that innate immune effectors are critical for effective host
defense. Initially, the innate and adaptive immune responses were thought to act
independently, with the innate response providing the first line of defense against invading
microbes, and the adaptive response being activated later to sterilize the infection. It is now
apparent that the adaptive response has co-opted many of the innate effector mechanisms to
enhance its effectiveness. Additionally, the adaptive immune system requires innate signals
for its activation. By using innate signals to help initiate its responses, the adaptive immune
system takes advantage of the innate systems ability to discriminate between contact with
dangerous pathogens and innocuous or even beneficial microbes and environmental factors.
This ability of the innate immune system to sense danger is essential for well-regulated
immune responses. Thus, the innate and adaptive arms of the immune response should be
viewed as complementary and cooperating.
Toll-Like Receptors
Toll was first identified in Drosophila where Toll was found to control polarity of the
developing embryo and later was recognized to participate in the flys anti-fungal immunity.
Cloning of Drosophila Toll showed that it encoded a transmembrane receptor whose
extracellular domain contained leucine-rich repeating units, while its cytoplasmic domain
had homology to the cytoplasmic domain of the IL-1 receptor of mammals (designated the
Toll/IL-1 Receptor domain, TIR). This suggested that there might be Toll homologues in
mammals. Indeed, 10 human Toll-like receptors (TLR) have now been defined. The TLR
appear largely to recognize pathogen-associated molecular patterns (PAMP).77 These
include LPS from Gram-negative bacteria, peptidoglycan, lipoteichoic acid,
lipoarabinomannan, bacterial flagellar proteins, viral double stranded RNA, and
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unmethylated DNA with CpG motifs characteristic of microbial DNA. TLR are particularly
found on macrophages and dendritic cells, but also are expressed on neutrophils,
eosinophils, epithelial cells, and keratinocytes. Although activation of some TLR can
activate or potentiate an allergic, Th2 type response, activation of most TLR elicits
mediators that program CD4 T cells towards a non-atopic Th1 response. TLR9, activated by
interaction with CpG DNA, provides the molecular basis for efforts to divert Th2-driven
atopic responses to non-atopic Th1 dominated responses.78 Downstream signal transduction
through most TLR is dependent on MyD88, a cytoplasmic protein encoded by the myeloid
differentiation primary response gene 88. MyD88 also mediates signaling through the IL-1
receptor. MyD88-defficiency leads to life threatening, recurrent pyogenic infections.79
Nucleotide-Binding Domain, Leucine-Rich Repeat (NLR) Proteins and the Inflammasome
All of the TLR proteins are transmembrane molecules, some expressed on the plasma
membrane of the cell where they can interact with extracellular triggering molecules, and
some expressed on intracellular membranes where they can interact with structures on
intracellular microbes and viruses. Another set of pattern recognition molecules, designated
NLR, has also been identified. These molecules are cytosolic and appear to interact with
soluble intracellular ligands. Like the TLR, the NLR are characterized by the presence of
leucine-rich repeat structures that are thought to contribute to their ability to bind to
conserved microbial structures. The NLR can also recognize endogenous signals of cellular
damage, such as uric acid crystals. Over 20 NLR-encoding genes have been identified in the
human genome. Most are characterized by the presence of a C-terminal leucine-rich repeat
domain that is thought to interact with microbial structures, a central nucleotide-binding
oligomerization domain that is used to form multimeric complexes of the NLR, and an Nterminal effector domains that allow the NLR to recruit a class of intracellular cysteine
proteinases (caspases) that activate the cellular apoptosis pathways or that activate the NFkB transcription factor to induce a broad pro-inflammatory response.80 One of the NLR
proteins, NALP3, has a special function in the innate immune response. Activation of
NALP3 leads to its association with the intracellular adapter protein that is designated
apoptosis-associated speck-like protein containing a caspase recruitment domain (ASC),
which combines with and activates caspase-1, leading to an active enzyme complex termed
the inflammasome. The inflammasome functions to activate the potent proinflammatory
molecules IL-1, IL-18, and IL-33.81 Recent studies have shown that alum, the most
common adjuvant in vaccines administered to humans, is taken up by phagocytic cells
where it activates NALP3, activating the inflammasome. This is crucial for its adjuvant
activity. If any one of NALP3, ASC, or caspase-1 is absent or defective, then alum can no
longer serve to augment the antibody response.82
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recognizes microbial carbohydrates, nuclear substances, and amyloid fibrils and thus
contributes to the host response to clear infections, autoimmunity and amyloidosis.85 The
ficolins contain CRD domains that share structure with fibrinogen.2 After binding to
carbohydrates on a microbe, they activate complement through the lectin pathway (see
below) and thus contribute importantly to clearance of the microbe.
Chitinases
The major phagocytic cells are neutrophils, macrophages, and monocytes. These cells engulf
pathogenic microbes and localize them in intracellular vacuoles were they are exposed to
toxic effector molecules such as nitric oxide, superoxide, and degradative enzymes in an
effort to destroy the organism. Phagocytic cells use a variety of Fc receptors and
complement receptors to enhance uptake of particles that have been marked by the adaptive
and innate immune systems for destruction.
Natural Killer (NK) Cells
NK cells are thought to represent a third lineage of lymphoid cells. When activated, they
have the morphology of a large granular lymphocyte. They develop in the bone marrow
under the influence of IL-2, IL-15, and bone marrow stromal cells. They represent only a
small fraction of peripheral blood cells and a small fraction of lymphoid cells in the spleen
and other secondary lymphoid tissues. NK cells have no antigen-specific receptors. Their
cytotoxic activity is inhibited by encounter with self-MHC molecules via inhibitory
receptors on their surface that recognize class I HLA molecules. They thus kill self cells that
have down-regulated class I molecule expression. This is important in host defense since
several viruses have developed mechanisms to down regulate class I expression in infected
cells as a strategy to avoid CD8+ cell killing. NK cells, however, also possess activating
receptors. The nature of the ligands for these receptors and the mechanisms by which they
contribute to identifying proper targets for NK cell cytotoxicity are currently under
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The complement system is a very important effector component of both adaptive and innate
immunity. The complement system is composed of over 25 plasma and cell surface proteins
that include three activation pathways and soluble and membrane bound down-modulating
regulatory pathways.91, 92 Many of the proteins of the activation pathway are proteinases,
and activation occurs in a cascade by proteolytic activation of one zymogen that then
activates the next zymogen in the pathway. The main goal of the activation pathway is to
mark targets permanently for destruction, to recruit other proteins and cells that facilitate
target destruction, and in the case of some bacteria and viruses to participate directly in the
destructive process by osmotic lysis. Antigen-antibody complexes provide the activating
signal for the Classical Pathway of Complement Activation. Sequential activation of
complement components C1, C4, and C2 produces the key enzyme in the pathway, the C3
convertase, which acts to cleave and activate C3. The cleavage results in release of the small
C3a fragment, a potent anaphylatoxin that induces mast cell degranulation, creates edema
and recruits phagocytic cells, and the larger C3b fragment which covalently attaches to the
activating antigen, marking it for destruction. C3b serves both as a site for attack of the
complement membrane attack complex (MAC), a self-assembling pore forming complex of
serum proteins that kills targets by osmotic lysis, and as an opsonin, enhancing phagocytosis
by its binding to complement receptors on the surfaces of neutrophils and macrophages.93
The second activation pathway, the Alternative Pathway of Complement Activation, is
activated without antibody by microbial structures that neutralize inhibitors of spontaneous
complement activation. This activation pathway can deposit >105 molecules of C3b on a
single bacterium in less than 5 minutes. C3b deposited in this way then triggers the MAC
and also enhances phagocytosis and killing.94
The third activation pathway is triggered by microbial cell wall components containing
mannans and is called the Lectin Pathway of Complement Activation.95 The interaction of
mannan-containing microbes with plasma mannan binding lectin (MBL) activates the
zymogenic plasma proteases MBL-associated serine proteases 1 and 2 (MASP-1, MASP-2).
These form a protease analogous to the activated C1 of the classical pathway that then goes
on to activate C4, C2 and the remainder of the pathway. The lectin pathway can also be
activated by complexes of microbes and host pentraxins and ficolins. Together, these three
activation pathways permit complement to participate in the destruction and clearance of a
wide variety of pathogens and macromolecules.
The effector mechanism of complement is potent and recruits intense local inflammation.
There are several plasma proteins (factor H, C4 binding protein) and membrane proteins
(complement receptors 14, decay accelerating factor, membrane co-factor protein) that
inhibit the complement activation pathways to prevent unwanted damage to host tissues.95
The importance of the activation and regulatory pathways of complement are underscored
by the dramatic phenotype of inherited deficiencies of individual components.91
Deficiencies of components of the MAC lead to increased susceptibility to infection with
Neisseria. Deficiency of C3 results in life threatening susceptibility to pyogenic infections,
often fatal during childhood. Deficiency of C4 or C2 causes a lupus-like immune complex
disease, indicating that one of the roles of the classical pathway is to participate in the host
response to and clearance of immune complexes. Deficiency of the serum inhibitor of C1
(an inhibitor of spontaneous activation of C1 and also of several components of the
J Allergy Clin Immunol. Author manuscript; available in PMC 2010 August 18.
Chaplin
Page 21
Rolling cells can then be induced to arrest and adhere firmly to the endothelium by
interactions between integrins on the leukocyte surface and Ig domain cell adhesion
molecules on the endothelial cells. Integrins are heterodimers of one and one chain. Key
integrins for leukocyte adhesion are LFA1 (CD11a/CD18, L2), VLA4 (CD49d/CD29,
41), and Mac-1 (CD11b/CD18, M2) that bind to the Ig domain cell adhesion molecules
ICAM-1, VCAM-1, and ICAM-1/C3b respectively. Binding of leukocytes to endothelial
cells is enhanced by the expression of chemokines by the endothelial cells or by underlying
damaged cells and tissues (see chapter 5).
Cellular Homeostasis
After an immune response is completed, the majority of antigen responsive cells must be
removed in order to prepare for the next immune challenge faced by the organism. Removal
of effector cells without causing inflammation and tissue damage is best achieved by
inducing the unwanted cells to undergo apoptosis. Molecules of the TNF family provide
strong signals for the apoptotic programmed cell death pathway. TNF, signaling through the
type I TNF receptor, induces death in tumor cells and at sites of ongoing inflammation. An
alternative apoptosis-inducing receptor, Fas, is more specifically involved in regulatory
apoptotic events. Fas, for example, transmits important apoptotic signals during thymic T
cell selection.50, 99 It also contributes to the regulation of autoreactive cells in the periphery.
100 Defects in Fas or in its ligand, FasL, result in autoimmune disorders with prominent
lymphoproliferation.101 Thus, deregulated Fas or its ligand may contribute importantly to
autoimmune diseases.
Chaplin
Page 22
cells and digested so as to eliminate both the potentially inflammatory contents of the
infected cell and also the microbe that was multiplying inside the cell.
Some degree of local inflammation is, however, often an important part of an effective host
immune response. The key elements of inflammation are part and parcel of the hosts
mobilization of its defense and repair responses. When inflammation is modest and
controlled, normal tissue architecture and function can be restored after the pathogen or
toxin has been eliminated. If the inflammatory response is excessively severe, however,
there is danger of lasting tissue damage, and the development of fibrosis during the
resolution of the inflammatory state.102 Mild fibrosis is physiological and generally does not
interfere with normal tissue function; however, when inflammation is either very severe or
becomes chronic the resulting fibrosis may lead to profound organ dysfunction. There has
been important progress over the last several years in understanding the mechanisms that
control the transition from physiologically appropriate inflammation and tissue repair to
damaging fibrosis. A common theme underlying the fibrotic process is the local production
of activated fibroblasts via the action of selected cytokines and other mediators on tissue
epithelial cells. Through the process of epithelial to mesenchymal transition, epithelial cells
are thought to be converted to activated fibroblasts and myofibroblasts that are then
responsible for the tissue changes that lead to fibrosis.103 Development of therapeutics that
target the mediators of tissue fibrosis may prevent many of the long-term complications of
chronic inflammation.
Perhaps more puzzling are conditions in which tissue inflammation appears to develop
without any underlying infectious or noxious stimulus. Prominent in these are autoimmune
diseases and atopic illnesses. These disorders appear to represent a fundamental misdirection
of the immune response, resulting in tissue damage when no real danger was present. The
growing spectrum of autoimmune diseases appears to represent a breakdown in selftolerance. This leads to the induction of both cellular and humoral immune responses against
components of self-tissues. Usually, both the cellular and humoral aspects of these
pathological responses have features of a Th1-type or Th17-type CD4 T cell response,
suggesting that defective regulation of either T cell differentiation or activation underlies the
response.104 Atopic diseases rarely manifest autoimmune character (although some forms of
chronic urticaria are thought to have an autoimmune etiology; see chapters 12 and 17).
Rather, they appear to represent an overly aggressive Th2 type response leading to
hypersensitivity to a broad spectrum of normally encountered environmental antigens.
Epidemiological studies have demonstrated that there is an inherited component to both the
autoimmune and the atopic diseases.105 There also appears to be a strong interplay with
environmental factors, perhaps including unrecognized infectious microbes or toxic agents
in the environment. The central role of Treg cells in controlling all aspects of the CD4 T cell
response, and the observation that congenital absence of Treg cells (as in the immune
dysregulation, polyendocrinopathy, enteropathy, X-linked [IPEX] syndrome) leads to
development of an aggressive autoimmune state106 suggest that disturbed Treg function may
underlie all autoimmune and atopic diseases. While disordered Th1, Th17 and Th2
responsiveness is a major manifestation of these illnesses, the disorders do not simply
represent a predisposition to over-polarization of the CD4+ T cell response. Epidemiological
studies have shown that the presence of atopy shows little protection against development of
the Th1/Th17-predominant illness rheumatoid arthritis.107 In fact, other studies have
suggested that patients with an autoimmune illness are more likely to have an atopic
disorder, suggesting that they have a common underlying etiology.108 Development of a
thorough understanding of the mechanisms underlying these two types of T cell-mediated
inflammation will lead to important new therapeutic options for successful treatment of
these common diseases.109
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Conclusion
NIH-PA Author Manuscript
The immune system uses many mechanisms to combat infection by microbes. These
mechanisms work together, and the fully integrated immune response draws elements from
many effector systems in order to tailor a response to the specific invading pathogen.
Abnormal regulation of the various effector mechanisms can lead to chronic or acute tissue
damage. Understanding the relationships between the different immune effector pathways
will permit improved immunomodulatory therapeutics, development of improved vaccines,
and avoidance of unintended tissue injury.
Abbreviations used
AID
AIRE
Autoimmune regulator
AMC
APC
APECED
ACS
Bf
Complement factor B
CD
Cluster of differentiation
CD40L
CD40 ligand
CFU
CLIP
CLP
Chitinase-like protein
CRD
CRP
C-reactive protein
DNA-PK
J Allergy Clin Immunol. Author manuscript; available in PMC 2010 August 18.
Chaplin
Page 24
DP
Double positive
ER
Endoplasmic reticulum
FcRI
FDC
Flt3
Foxp3
Forkhead box P3
GM-CSF
HLA
Human leukocyte-associated
HLDA
IFN
Interferon
Ig
Immunoglobulin
Ii
Invariant chain
IL
Interleukin
IPEX
ITAM
Jak
Janus kinase
LPS
Lipopolysaccharide
MAC
MAP
Mitogen-associated protein
MASP
MBL
MHC
MIC
MyD88
NK
Natural killer
NLR
PAMP
PD-1
Programmed death-1
PD-L1
Programmed death-ligand 1
RAG
Recombinase-activating gene
SCID
STAT
TAP
Tc
T cytotoxic
TCR
T cell receptor
TdT
J Allergy Clin Immunol. Author manuscript; available in PMC 2010 August 18.
Chaplin
Page 25
TGF
Th
T helper
TIR
Toll/IL-1 receptor
TLR
Toll-like receptor
TNF
Treg
T regulatory
TSLP
TSST-1
UNG
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Pluripotent hematopoietic stem cells differentiate in bone marrow into common lymphoid or
common myeloid progenitor cells. Lymphoid stem cells give rise to B cell, T cell, and NK
cell lineages. Myeloid stem cells give rise to a second level of lineage specific colony form
unit (CFU) cells that go on to produce neutrophils, monocytes, eosinophils, basophils, mast
cells, megakaryocytes, and erythrocytes. Monocytes differentiate further into macrophages
in peripheral tissue compartments. Dendritic cells (DC) appear to develop primarily from a
DC precursor that is distinguished by its expression of the Flt3 receptor. This precursor can
derive from either lymphoid or myeloid stem cells and gives rise to both classical DC and
plasmacytoid DC. Classical DC can also derive from differentiation of monocytoid
precursor cells. Modified with permission from Huston.114
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The human MHC, designated HLA, is encoded on the short arm of chromosome 6. The
locations of the major HLA and related genes are shown above a scale showing approximate
genetic distances in kilobase pairs of DNA (kbp). The genes encoding the Class I HLA
heavy chains (shown in blue) are clustered at the telomeric end of the complex. The genes
encoding the Class II HLA and chains (shown in green) plus the genes encoding the
LMP1/2, TAP1/2, and Tapascin (TAPBP) molecules (shown in orange) are clustered at the
centromeric end of the complex. In between the Class I and the Class II genes are additional
genes designated Class III (shown in red). These include genes encoding the cytochrome
P450 21-hydroxylase (CYP21B), an inactive cytochrome P450 pseudogene (CYP21Ps),
complement components C4, C2 and factor B (Bf), tumor necrosis factor (TNF), and the two
lymphotoxin chains (LTA, LTB). There are two isoforms of complement C4 designated
C4A and C4B. C4A interacts more efficiently with macromolecules containing free amino
groups (protein antigens), whereas C4B interacts more efficiently with macromolecules
containing free hydroxyl groups (glycoproteins and carbohydrates). There are genes
encoding two additional HLA Class I-like molecules designated MICA and MICB (shown
in purple) located between the Class III genes and the classical Class I genes. Nonfunctional pseudogenes are shown in gray and further designated by italics.
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Molecular models derived from crystal structures of class I (AC) and class II (DF) HLA
molecules. A, the class I 1, 2, and 3 domains are shown (light blue) in non-covalent
association with the 2m molecule. Coils represent -helices, and broad arrows represent strands. Anti-parallel -strands interact to form -sheets. The -helices in the 1 and 2
domains form the sides and floor of a groove that binds processed antigenic peptides
(yellow). The transmembrane and intracytoplasmic portions of the heavy chain are not
shown. B, top view of the 1 and 2 domains displaying the antigenic peptide in a molecular
complex for recognition by the TCR of a CD8+ T cell (recognition site outlined by pink
rectangle). C, side view of the 1 and 2 domains highlighting the TCR contact points on
both the -helices and antigenic peptide. D, side view of the HLA class II molecule showing
the chain (light blue) and the chain (dark blue). In the class II protein, the peptidebinding groove is made of helices in both the 1 and 1 domains and a -sheet formed
again by both the 1 and 1 domains. E, top view of the both the 1 and 1 domains and the
processed antigenic peptide fragment as they would be seen by the TCR of a CD4+ T cell. F,
side view highlighting the 1 and 1 domains and the antigenic peptide. Modified with
permission from Bjorkman.16
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In the endoplasmic reticulum (ER), newly synthesized class II proteins associate with the
help of calnexin with an invariant chain protein that protects the antigen-binding groove of
the class II molecule until it is transported to the class II+ endosomal protein loading
compartment. Exogenous antigens are taken up by phagocytosis or endocytosis, digested by
the action of lysosomal enzymes, and transported to the class II+ peptide loading
compartment for loading into a class II protein. There the invariant chain is proteolytically
degraded and replaced by antigenic peptide with the help of the HLA-DM protein. The
assembled class II protein-peptide complex is then delivered to the plasma membrane for
recognition by CD4+ T cells. Modified with permission from Huston.114
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Hematopoietic stem cells which do not express CD3, CD4 or CD8 but which are committed
to T cell differentiation move from the bone marrow to the thymic subcapsular zone. There
they begin rearrangement of the TCR genes. Once a productive TCR chain has been
produced, they move the thymic cortex where TCR chain rearrangement occurs and
surface expression of the CD3, CD4 and CD8 proteins is induced. These CD4+CD8+
(double positive) cells are positively selected on cortical epithelial cells for their ability to
recognize self Class I or Class II HLA proteins. If the developing T cell has adequate
affinity to recognize a self Class I protein, then it retains expression of CD8 and
extinguishes expression of CD4. If the cell recognizes a self Class II protein, then it retains
expression of CD4 and extinguishes expression of CD8. Selected CD4/CD8 single positive
(SP) cells then move to the thymic medulla where they are negatively selected on medullary
epithelial cells to remove cells with excessive affinity for self-antigens presented in HLA
molecules. Cells emerge from positive selection SP for CD4 or CD8 expression and then are
exported to the periphery. Cells that fail positive or negative selection are removed by
apoptosis. A small fraction of cells differentiate from to rearrange their TCR and chains,
rather than their TCR and chains. Modified with permission from Huston.114
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A, the complete TCR complex includes the rearranged TCR and chains and also the
CD3, CD3, CD3, and CD3 chains. The CD3 chains contain ITAMs in their cytoplasmic
domains that can be phosphorylated to activate the intracellular signaling cascade for T cell
activation. The signaling protein tyrosine kinases Lck and Fyn associate with the
intracellular portions of the CD4 and CD3 chains respectively. TCR engagement by MHC
plus peptide without the presence of costimulatory proteins fails to activate phosphorylation
of the CD3 ITAMs and results in anergy. B, TCR engagement by MHC plus peptide with
costimulatory interactions between CD28 on the T cell and CD80 or CD86 (B7.1 or B7.2)
on the APC results in Lck- and Fyn-dependent phosphorylation of the CD3 chains, and
recruitment of the adapter protein ZAP-70 to the CD3 complex. This leads to
phosphorylation of ZAP-70, which induces the downstream program of T cell activation. C,
polyclonal activation of T cells can be elicited by superantigens which interact outside the
peptide binding groove with the 1 chain of the class II molecule and with all V chains of a
particular subclass. This activates CD4-independent, but Fyn-dependent phosphorylation of
the CD3 chains, recruitment and phosphorylation of ZAP-70, and cell activation.
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B cells differentiate in the bone marrow from stem cells to become mature surface IgM and
IgD expressing cells. This occurs in the absence of antigen. In peripheral lymphoid tissues,
the B cell can then mature further under the influence of antigen and T cell help to undergo
isotype switching and affinity maturation by somatic mutation. The factors controlling the
final differentiation from antibody-secreting B cell to plasma cell are incompletely
characterized, but require the participation of the transcription factors Blimp1, Xbp1 and
IRF4. Correlations are show between the stage of cell differentiation and the expression of
key molecules in the cell (TdT, RAG1/RAG2, cytoplasmic ) and on the cell surface (class
II, CD19, CD21, CD25, CD45, and surface Ig). Modified with permission from Huston.114
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C3b on the activating microbial particle or immune complex. This opsonizes the particle for
phagocytosis and initiates the activation of the membrane attack complex. The C5a fragment
that is proteolytically released from C5 also is a highly anaphylatoxic molecule that induces
intense local inflammation.
Molecular
Weight, kDa
Concentration
In Serum, mg/ml
Complement
Activating C/A2
Macrophage
FcR Binding
Mast Cell
Sensitizing
Placental
Transport
Mucosal
Transport3
/+
0.03
175
IgD
++
++
++/+
10
150
IgG1
Dimer only
Subunit
Form1
IgM
++
+/+
150
IgG2
++
++
++/+
150
IgG3
+/
/+
0.5
150
IgG4
+++
++
/+
160,400
1,2
IgA1
+++
++
/+
0.5
160,400
1,2
IgA2
+++
0.003
190
IgE
Table I
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