Location via proxy:   [ UP ]  
[Report a bug]   [Manage cookies]                
Scribd Logo
Upload

Welcome to Scribd!

  • 855 views

    Tissue Processing

    Uploaded by

    Malliga Sundareshan
    This document provides an overview of the tissue processing techniques used to prepare tissues for microscopic examination. The most common technique is the paraffin method, which involves fixing tissues, dehydrating them using increasing concentrations of alcohol, clearing them using xylene, and embedding them in paraffin wax. This allows thin sections to be cut for microscopic analysis. Alternative techniques like freezing or embedding in plastics are also discussed briefly. The goal of tissue processing is to firm tissues so they can be thinly sectioned for diagnostic examination under the microscope.

    Copyright:

    © All Rights Reserved
    Download as PPT, PDF, TXT or read online from Scribd

    Tissue Processing

    Uploaded by

    Malliga Sundareshan
    855 views34 pages
    This document provides an overview of the tissue processing techniques used to prepare tissues for microscopic examination. The most common technique is the paraffin method, which involves fixing tissues, dehydrating them using increasing concentrations of alcohol, clearing them using xylene, and embedding them in paraffin wax. This allows thin sections to be cut for microscopic analysis. Alternative techniques like freezing or embedding in plastics are also discussed briefly. The goal of tissue processing is to firm tissues so they can be thinly sectioned for diagnostic examination under the microscope.

    Original Description:

    processing of tissues

    Copyright

    © © All Rights Reserved

    Available Formats

    PPT, PDF, TXT or read online from Scribd

    Did you find this document useful?

    Is this content inappropriate?

    This document provides an overview of the tissue processing techniques used to prepare tissues for microscopic examination. The most common technique is the paraffin method, which involves fixing tissues, dehydrating them using increasing concentrations of alcohol, clearing them using xylene, and embedding them in paraffin wax. This allows thin sections to be cut for microscopic analysis. Alternative techniques like freezing or embedding in plastics are also discussed briefly. The goal of tissue processing is to firm tissues so they can be thinly sectioned for diagnostic examination under the microscope.

    Copyright:

    © All Rights Reserved
    Download as PPT, PDF, TXT or read online from Scribd
    Download as ppt, pdf, or txt
    855 views34 pages

    Tissue Processing

    Uploaded by

    Malliga Sundareshan
    This document provides an overview of the tissue processing techniques used to prepare tissues for microscopic examination. The most common technique is the paraffin method, which involves fixing tissues, dehydrating them using increasing concentrations of alcohol, clearing them using xylene, and embedding them in paraffin wax. This allows thin sections to be cut for microscopic analysis. Alternative techniques like freezing or embedding in plastics are also discussed briefly. The goal of tissue processing is to firm tissues so they can be thinly sectioned for diagnostic examination under the microscope.

    Copyright:

    © All Rights Reserved
    Download as PPT, PDF, TXT or read online from Scribd
    Download as ppt, pdf, or txt
    of 34

    Tissue Processing

    Presented by: Walaa Mal


    Histopathology teaching
    assistant

    Contents

    Introduction
    Specimen Accessioning
    Gross Examination
    Tissue Processing steps
    The paraffin Technique and its alternatives
    The freezing Technique

    Problems in tissue processing

    Introduction
    There are 3 main techniques which are used in
    preparing microscopical sections from tissues:
    The paraffin technique (It is the most common method)
    The celloidin technique (It is the most perfect method)
    The freezing technique (It is the most rapid method)

    Introduction
    Tissues from the body taken for diagnosis of disease
    processes must be processed in the histology
    laboratory to produce microscopic slides that are
    viewed under the microscope by pathologists.
    The techniques for processing the tissues, whether
    Biopsies,
    Larger specimens removed at surgery, Or
    Tissues from autopsy are described below.

    The persons who do the tissue processing and make


    the glass microscopic slides are
    HISTOTECHNOLOGISTS.

    Specimen Accessioning

    Tissue specimens received in the surgical


    pathology laboratory have a request form
    that lists the patient information and
    history along with a description of the
    site of origin.
    The specimens are accessioned by giving
    them a number that will identify each
    specimen for each patient.

    Gross examination

    Tissues removed from the body for diagnosis


    arrive in the Pathology Department and are
    examined by a pathologist, pathology assistant, or
    pathology resident.
    Gross examination consists of describing the
    specimen and placing all or parts of it into a
    small plastic cassette which holds the tissue
    while it is being processed to a paraffin block.
    Initially, the cassettes are placed into a fixative.

    Gross examination
    Note:
    When a malignancy is suspected, then the
    specimen is often covered with ink in order
    to mark the margins of the specimen.
    Different colored inks can be used to identify
    different areas if needed.
    When sections are made and processed, the
    ink will mark the actual margin on the slide.

    Tissue Processing steps

    Biological tissues are generally rather soft,


    making it quite difficult to cut acceptably thin
    sections directly from the fresh or fixed tissues.
    Methods must be used to hold the tissues firm,
    which facilitates cutting thin sections with a
    sharp knife.
    Firmness can be achieved either by embedding
    the tissues in a suitable embedment or by
    freezing the tissue.
    Once the tissue has been fixed, it must be
    processed into a form in which it can be made
    into thin microscopic sections.

    Tissue Processing steps

    The usual way this is done is with paraffin.


    Tissues embedded in paraffin, which is
    similar in density to tissue, can be sectioned
    at anywhere from 3 to 10 microns, usually
    5-8 routinely.
    The technique of getting fixed tissue into
    paraffin is called tissue processing.
    The main steps in this process are
    dehydration and clearing.

    The paraffin Technique


    Washing
    Following fixation, the tissues should
    be washed from 15 to 30 minutes. The
    fixed tissues are washed in running tap
    water to remove the fixative from
    them.

    ...The paraffin Technique

    Dehydration
    Wet fixed tissues (in aqueous solutions) cannot be directly
    infiltrated with paraffin.
    First, the water from the tissues must be removed by dehydration.
    This is usually done with a series of alcohols; say 70% to 95% to 100%.
    The organic solvent must replace the water gradually to prevent turbulence
    at the interface between water and pure ethanol
    Turbulence could cause damage or distortion to cellular components.
    The number of steps or the gradient differences should be determined by

    The degree of fixation


    The delicacy of the tissue
    The degree of cellular detail to be preserved

    Sometimes the first step is a mixture of formalin and alcohol.


    Other dehydrants can be used, but have major disadvantages.
    Acetone is very fast, but a fire hazard, so is safe only for small, handprocessed sets of tissues.
    Dioxane can be used without clearing, but has toxic fumes.

    The paraffin technique


    Clearing
    The next step is called "clearing" and consists of removal
    of the dehydrant with a substance that will be miscible
    with the embedding medium (paraffin).
    The commonest clearing agent is xylene.
    Toluene works well, and is more tolerant of small amounts of
    water left in the tissues, but is 3 times more expensive than
    xylene.
    Chloroform used to be used, but is a health hazard, and is
    slow.
    Methyl salicylate is rarely used because it is expensive, but it
    smells nice (it is oil of wintergreen).
    Excessive exposure to clearing reagents may cause excessive
    hardness or shrinkage.

    The paraffin technique


    Impregnation in paraffin
    The tissues are put from 6 24 hours in hot
    soft paraffin at 50C, then in hot hard
    paraffin at 55 C in the oven. The paraffin will
    penetrate in-between the cells of the tissues.
    This process of paraffin infiltration is a
    necessary step to harden the tissues before
    their embedding.

    The paraffin technique


    Embedding
    Finally, the tissue is infiltrated with the embedding agent,
    almost always paraffin.
    In early days of microscopy histologists tried to harden tissues
    artificially with fixatives, in order to be able to cut suitably thin sections
    for microscopy.
    Nearly 100 years ago, the method of embedding tissues in paraffin
    was developed
    Paraffin is a derivative of crude petroleum. It is a group of variable
    length, long-chain hydrocarbons of the methane series
    Most paraffins suitable as embedding media melt between 52 and
    58C.
    Since most paraffin have a melting point between 52-58C, it must
    infiltrate the cells while it is hot.

    The paraffin technique

    Infiltration must be carried out at only a few


    degrees above the melting point of paraffin
    This represented a great step forward in
    microscopic techniques.
    Firmness was achieved with a supporting
    medium (an embedment), rather than by
    hardening the tissue itself.
    For many years paraffin served as almost the only
    embedment.
    Most of our knowledge from microscopy has
    been gained from sections cut from paraffinembedded tissues.

    The paraffin technique

    Paraffin can be purchased that differ in melting point, for various


    hardnesses, depending upon the way the histotechnologist likes them
    and upon the climate (warm vs. cold).
    Recently a product called Paraplast Plus was introduced into the
    market. It contains added plasticizers that make the paraffin blocks
    easier for some technicians to cut.
    A vacuum can be applied inside the tissue processor to assist
    penetration of the embedding agent.
    The time required for embedding tissues using ethanol dehydration
    and xylene clearing usually exceeds eight hours.
    Normally, the tissue is processed overnight with an automatic tissue
    processing machine.

    The paraffin technique

    Using a completely different rationale for dehydration,


    Prento (1978) was able to reduce the time required for
    embedding fixed tissues to less than 3 hours, using far
    few steps.
    He used Dimethoxypropane (DMP), which served as
    both the dehydrating and clearing agent.
    Acidified DMP does not simply replace the water but
    chemically reacts with water to form methanol and acetone
    which both act as dehydrants.
    After the block of tissue has been completely infiltrated
    with paraffin, it is placed in a mold containing hot
    paraffin and oriented in the desire manner.
    The paraffin is then allowed to solidify.

    The paraffin technique

    Upon solidifying, paraffin shrinks 16.5 percent in volume.


    Paraplast is supposed to shrink less (14 percent by volume)
    No doubt the two most objectionable aspects of
    paraffin as an embedding medium are:

    The heat required for melting- the critical shrinkage point of


    collagen is approximately 65C. Exposure of collagenous tissues to
    this temperature must be carefully guarded against to avoid
    excessive shrinkage.
    Shrinkage upon solidification

    Despite these problems, paraffin has been far the most


    widely used embedding medium for many years, and it will
    probably not be readily replaced by another medium.

    The paraffin technique


    The above processes are almost always automated
    for the large volumes of routine tissues processed.
    Automation consists of an instrument that moves
    the tissues around through the various agents on a
    preset time scale.
    The "technicon" tissue processor is one of the
    commonest and most reliable (a mechanical
    processor with an electric motor that drives gears
    and cams), though no longer made.
    Newer processors have computers, not cam wheels,
    to control them and have sealed reagent wells to
    which a vacuum and/or heat can be applied.

    The paraffin technique


    Tissues that come off the
    tissue processor are still
    in the cassettes and must
    be manually put into the
    blocks by a technician
    who must pick the tissues
    out of the cassette and
    pour molten paraffin
    over them. This
    "embedding" process is
    very important, because
    the tissues must be
    aligned, or oriented,
    properly in the block of
    paraffin.

    Alternatives to paraffin embedding

    Alternatives to paraffin embedding include various plastics that


    allow thinner sections. Such plastics include:
    Methyl Methacrylate,
    Glycol Methacrylate (GMA),
    Araldite
    Epon.
    Methyl Methacrylate is very hard and therefore good for
    embedding undecalcified bone.
    Glycol Methacrylate has the most widespread use since it is the
    easiest to work with.
    Araldite is about the same as methacrylate, but requires a more
    complex embedding process.
    Epon is routinely used for electron microscopy where very thin
    sections are required

    Note:
    Plastics require special reagents for
    dehydration and clearing that are expensive.
    For this reason, and because few tissues are
    plastic embedded, the processing is usually done
    by hand.
    A special microtome is required for sectioning
    these blocks.
    Small blocks must be made, so the technique
    lends itself to small biopsies, such as bone
    marrow or liver.

    The freezing Technique


    In this method, the fresh or fixed tissues are frozen hardened
    and cut with a freezing microtome in the cryostat apparatus
    within few minutes
    It is a quick and simple method which is commonly used
    during operations for rapid diagnosis of tumors e.g.
    carcinoma
    The chemistry of tissues is preserved because we use no heat
    and no chemical solvents
    Can be used in Histochemistry to demonstrate enzymes and
    chemical components of tissues
    Disadvantage: It gives not-serial thick sections which may
    fragment into small pieces, so they are very difficult to be
    stained and to be stored.

    Problems in Tissue Processing

    "Floaters" are small pieces of tissue that appear


    on a slide that do not belong there--they have
    floated in during processing.
    Floaters may arise from sloppy procedure on
    the cutting bench-- dirty towels,
    instruments, or gloves can have tissue that is
    carried over to the next case.
    Therefore, it is essential that you do only one
    specimen at a time and clean thoroughly before
    opening the container of the next case.

    Problems in Tissue Processing

    If reusable cassettes are employed, you must be aware


    that tissue may potentially be carried over and appear as
    "floaters" even several days later, when the cassette is reused.
    The problem arises when, during embedding, not all the
    tissue is removed from the cassette. Then, in the cleaning
    process, not all of the wax is removed. Then, the next
    person using the cassette does not pay attention to the
    fact that there is tissue already in the cassette and puts his
    specimen in it.
    The floater that appears on the slide will look wellpreserved--it should, because it was processed to paraffin.

    Problems in Tissue Processing

    Always be sure that you properly


    identify the tissue! This means that you
    make sure that the patient label on the
    specimen container matches that of the
    request slip.
    An accession number is given to the
    specimen. This number must appear with
    the tissue at all times.
    You must never submit a cassette of
    tissue without a label.

    Problems in Tissue Processing

    You must never submit a cassette of


    tissue with the wrong label.
    Mislabelling or unlabelling of tissues is
    courting disaster

    Sectioning
    Frozen Sections
    Staining
    H & E staining
    Coverslipping
    Decalcification
    Artefacts in Histologic Sections

    You might also like