1 Semen Analysis Learning Objectives Upon completion of this chapter the student will be able to: State the structures involved in sperm production and their function.
Describe the four components of semen with regard to source
and function.
Describe the normal appearance of semen and three
abnormalities in appearance.
State two possible causes of low semen volume.
Discuss the significance of semen liquefactionand viscosity.
2 Semen Analysis Learning Objectives cont..
Calculate a sperm concentration and count
Define round cells, and explain their significance.
Describe the appearance of normal sperm, including structures
and their functions.
Differentiate between routine and strict criteria for evaluation of
sperm morphology.
Given an abnormal result in the routine semen analysis, determine
additional tests that might be performed.
3 Semen Analysis Physiology
Semen is composed of four fractions that are
contributed by the testes, epididymis, seminal vessels, prostate, and bulbourethral glands.
Each fraction differs in its composition, and the mixing
of all four fractions during ejaculation is essential for the production of a normal semen specimen
4 Semen Analysis 5 Semen Analysis 1. Testes Germ cells for the production of spermatozoa are located in the epithelial cells of the seminiferous tubules of the testes.
Specialized Sertoli cells provide support and
nutrients for the germ cells as they undergo mitosis and meiosis (spermatogenesis).
When spermatogenesis is complete, the immature
sperm (nonmotile) enter the epididymis.
6 Semen Analysis In the epididymis, the sperm mature and develop flagella; stored until ejaculation.
During ejaculation they are propelled through
the ductus deferens (vas deferens) to the ejaculatory ducts.
7 Semen Analysis 2. Ejaculatory Ducts Receive both the sperm from the vas deferens and fluid from the seminal vesicles.
The seminal vesicles produce the majority of the fluid
present in semen (60% to 70%). The fluid contains a high concentration of fructose.
Spermatozoa metabolize the fructose for the energy
needed for the flagella to propel them through the female reproductive tract.
In the absence of fructose, sperm do not display motility in
the semen analysis.
8 Semen Analysis 3. Prostate Gland
The muscular prostate gland, surrounds the upper
urethra and aids in propelling the sperm through the urethra by contractions during ejaculation.
Approximately 20% to 30% of the semen volume is
acidic fluid produced by the prostate gland.
The acidic fluid contains high concentrations of ACP,
citric acid, zinc, and proteolytic enzymes responsible for both the coagulation and liquefaction of the semen following ejaculation.
9 Semen Analysis 4. Bulbourethral Glands
Contribute about 5% of the fluid volume in
the form of a thick, alkaline mucus helps to neutralize acidity from the prostate secretions and the vagina.
It is important for semen to be alkaline to
neutralize the vaginal acidity present as a result of normal bacterial vaginal flora.
Without this neutralization, sperm motility
would be diminished.
10 Semen Analysis Semen Analysis The beginning of the evaluation of reproductive dysfunction (infertility) in the male; b/c it is a cost-effective and relatively simple procedure.
Can also be used to select donors for therapeutic
insemination
Can also be used to monitor the success of surgical
procedures, such as varicocelectomy and vasectomy.
Used for forensic purpose like to determine whether
semen is actually present in a specimen, a primary example is in cases of alleged rape.
11 Semen Analysis Collection and transport of semen
The variety in the composition of the semen fractions
makes proper collection of a complete specimen essential for accurate evaluation of male fertility.
The majority of sperm are contained in the first
portion of the ejaculate, making complete collection essential for accurate testing of both fertility and postvasectomy specimens.
Patients should receive detailed instructions for
specimen collection.
12 Semen Analysis Specimens are collected following a period of sexual abstinence of from 2 to 3 days to not longer than 5 days.
Specimens collected following prolonged abstinence tend to
have higher volumes and decreased motility.
When performing fertility testing, 2 or 3 samples
are usually tested at 2-week intervals, with 2 abnormal samples considered significant.
The laboratory should provide warm sterile glass
or plastic containers.
13 Semen Analysis Whenever possible, the specimen is collected in a room provided by the laboratory. However, if this is not appropriate, the specimen should be kept at room temperature and delivered to the laboratory within 1 hour of collection.
Laboratory personnel must record the time of
specimen collection and specimen receipt.
Specimens awaiting analysis should be kept at
370C.
14 Semen Analysis Specimens should be collected by masturbation.
If this is not possible, only non-lubricant-containing
rubber or polyurethane condoms should be used.
Ordinary condoms are not acceptable because they have
spermicidal properties.
All semen specimens are potential reservoirs for
infectious pathogens (e.g. HIV and hepatitis viruses), and must be handled as potentially hazardous specimen during the analysis.
15 Semen Analysis Tests for semen When investigating male infertility, the basic semen analysis usually includes:
Measurement of volume, appearance, viscosity, liquefaction
Measurement of pH
Sperm count
Examination of a wet preparation
to estimate % motility & viability of sperm to look for cells and bacteria
Examination of a stained preparation to estimate the percentage of
spermatozoa with normal morphology.
16 Semen Analysis 1. Appearance Examination
Normal semen has a gray-white color, appears
translucent, and has a characteristic musty odor.
Increased white turbidity indicates the presence of
WBCs & infection within the reproductive tract.
During the microscopic examination, WBCs must be differentiated
from immature sperm (spermatids).
The leukocyte esterase reagent strip test may be useful to screen
for the presence of WBCs.
17 Semen Analysis Red coloration are associated with the presence of RBCs and are abnormal.
Yellow coloration may be caused by urine
contamination, specimen collection following prolonged abstinence, and medications.
Urine is toxic to sperm, thereby affecting the evaluation of motility.
18 Semen Analysis 2. Liquefaction
A fresh semen specimen is clotted and should
liquefy within 30 to 60 minutes after collection
Recording the time of collection is essential for evaluation of
semen liquefaction.
Analysis of the specimen cannot begin until
after liquefaction has occurred.
19 Semen Analysis If after 2 hours the specimen has not liquified, proteolytic enzymes such as alpha-chymotrypsin may be added to allow the rest of the analysis to be performed.
Failure of liquefaction to occur may be caused by a
deficiency in prostatic enzymes and should be reported.
20 Semen Analysis 3. Viscosity
Incompletely liquefied semen specimens are
clumped and highly viscous.
Increased viscosity and incomplete liquefaction
impede sperm motility.
21 Semen Analysis The normal semen specimen should be easily drawn into a pipette and form droplets that do not appear clumped or stringy when discharged from the pipette.
Semen droplets with threads longer than 2 cm are
considered highly viscous.
Ratings of 0 (watery) to 4 (gel-like) can be assigned to the
viscosity report.
Viscosity can also be reported as low, normal, and high.
22 Semen Analysis 4. Volume
Normal semen volume ranges b/n 2 & 5 mL.
Increased volume may be seen following periods
of extended abstinence.
Decreased volume is more frequently associated
with infertility and
May indicate improper functioning of one of the semen-
producing organs, primarily the seminal vesicles.
Incomplete specimen collection must also be considered.
23 Semen Analysis 5. PH
The normal pH of semen is alkaline (7.2 - 8.0).
Increased pH is indicative of infection within the
reproductive tract.
A decreased pH is associated with increased
prostatic fluid. Decreased PH and absence of sperm may indicate dysgenesis (failure to develop) of the vas deferens, seminal vesicles or epididymis. Semen pH testing can be done by urinalysis reagent strip; dedicated pH testing paper also can be used.
24 Semen Analysis Sperm Count
Even though fertilization is accomplished by one
spermatozoon, the actual number of sperm present in a semen specimen is a valid measurement of fertility.
Normal sperm counts are > 20 million sperm/ml
borderline b/n 10 - 20 million/ml
Sperm count is usually performed using the Neubauer
counting chamber; in the same manner as cells in the CSF.
25 Semen Analysis 26 Semen Analysis Dilution of the semen is essential because it immobilizes the sperm prior to counting.
The traditional diluting fluid contains sodium
bicarbonate and formalin, which immobilize and preserve the cells; however, good results can also be achieved using saline and distilled water.
The addition of stain, such as crystal violet, to the
diluting fluid aids in visualization when using bright- field microscopy.
27 Semen Analysis Only fully developed sperm should be counted.
Immature sperm and WBCs must not be included.
Their presence can be significant, and they may need to be identified and counted separately.
The presence of more than 1 million spermatids/ml indicates
disruption of spermatogenesis. This may be caused by viral infections, exposure to toxic chemicals, and genetic disorders.
Stain included in the diluting fluid aids in
differentiation b/n spermatids & WBCs, and they can be counted in the same manner as mature sperm.
28 Semen Analysis Sperm Motility
The presence of sperm capable of forward,
progressive movement is critical for fertility
b/c once presented to the cervix, the sperm must propel
themselves through the cervical mucosa to the uterus, fallopian tubes, and ovum.
29 Semen Analysis Estimate the percentage of motile spermatozoa Place 1 drop (~10-15µL) of well-mixed liquefied semen on a slide and cover with cover glass.
Focus the specimen using the 10x objective.
Ensure the spermatozoa are evenly distributed (if not,
re-mix the semen and examine a new preparation).
Using the 40x objective, examine several fields to
assess motility Motility can be excellent (rapid and progressive) or weak (slow and non-progressive).
30 Semen Analysis Sperm Motility Grading
31 Semen Analysis Count a total of 100 spermatozoa, and note out of the hundred how many are motile.
Record the percentage that are motile and nonmotile.
Normally over 50% of spermatozoa are motile within 60
minutes of ejaculation.
When more than 60% of spermatozoa are nonmotile,
examine an eosin preparation to assess whether the spermatozoa are viable or non-viable
32 Semen Analysis Sperm viability
Decreased sperm viability may be suspected when a
specimen has a normal sperm concentration with markedly decreased motility.
Viability is evaluated by mixing the specimen with an
eosin-nigrosin stain, preparing a smear, and counting the number of dead cells in 100 sperm.
Living cells are not infiltrated by the dye and remain a
bluish white color, whereas dead cells stain red against the purple background.
Normal viability requires 75% living cells and should
correspond to the previously evaluated motility.
33 Semen Analysis Sperm Morphology The presence of sperm that are morphologically incapable of fertilization also results in infertility.
Sperm morphology is evaluated with respect to
the structure of the head, neckpiece, midpiece, and tail.
Abnormalities in head morphology are associated
with poor ovum penetration, whereas neckpiece, midpiece, and tail abnormalities affect motility.
34 Semen Analysis The normal sperm has an oval- shaped head approximately 5µ m long and 3µ m wide and about 45µm long flagellar tail
Critical to ovum penetration is the
enzyme containing acrosomal cap located at the tip of the head.
The acrosomal cap should
encompass approximately half of the head and covers appproximately twothirds of the sperm nucleus. 35 Semen Analysis The neckpiece attaches the head to the tail and the midpiece.
The midpiece is the thickest part of the tail
because it is surrounded by a mitochondrial sheath that produces the energy required by the tail for motility.
36 Semen Analysis Sperm morphology is evaluated from a thinly smeared, stained slide under oil immersion. Staining can be performed using Wright’s, Giemsa, or Papanicolaou stain. Air-dried slides are stable for 24 hours.
At least 200 sperm should be evaluated and the
percentage of abnormal sperm reported.
Abnormal sperm tails are often doubled, coiled, or
bent
Routinely abnormalities in head structure include
double heads, pinheads,
giant and amorphous heads, tapered heads Constricted heads 37 Semen Analysis 38 Semen Analysis 39 Semen Analysis Seminal Fluid Fructose Low sperm concentration may be caused by lack of the support medium produced in the seminal vesicles.
can be indicated by a low to absent fructose level in the
semen.
Specimens can be screened for the presence of
fructose using the resorcinol test that produces an orange color when fructose is present.
40 Semen Analysis A normal quantitative level of fructose is equal to or greater than 13 µmol per ejaculate.
This can be determined using spectrophotometric methods.
Specimens for fructose levels should be tested within 2 hours or frozen to prevent fructolysis.
41 Semen Analysis Antisperm Antibodies
They can be present in both men and women.
They may be detected in semen, cervical mucosa,
or serum and are considered a possible cause of infertility.
It is not unusual for both partners to demonstrate
antibodies, although male antisperm antibodies are more frequently encountered.
42 Semen Analysis Under normal conditions, the blood-testes barrier separates sperm from the male immune system.
When this barrier is disrupted, as can occur following
surgery, trauma, and infection, the antigens on the sperm produce an immune response that damages the sperm.
The damaged sperm may cause the production of
antibodies in the female partner.
43 Semen Analysis The presence of antibodies in a male subject can be suspected when clumps of sperm are observed during a routine semen analysis.
The presence of antisperm antibodies in a female
subject results in a normal semen analysis accompanied by continued infertility.
The presence of antisperm antibodies in women may
be demonstrated by mixing the semen with the female cervical mucosa or serum and observing for agglutination.
A variety of immunoassay kits are available for both
semen and serum testing
44 Semen Analysis Microbial and Chemical Testing The presence of more than 1 million WBCs/ml indicates infection within the reproductive system, frequently the prostate.
Routine aerobic and anaerobic cultures most
frequently performed include tests for Chlamydiatrachomatis Mycoplasma hominis, and Ureaplasma urealyticum
45 Semen Analysis Chemical testing performed on semen may include determination of the levels of neutral-glucosidase zinc citric acid prostatic acid phosphatase (PAP)
Decreased neutral-glucosidase suggests a
disorder of the epididymis.
Decreased zinc, citrate, and acid phosphatase
indicate a lack of prostatic fluid
46 Semen Analysis On certain occasions, laboratories determine whether semen is actually present in a specimen (forensic purpose). A primary example is in cases of alleged rape.
Microscopically examining the specimen for the presence of sperm may
be possible, with the best results being obtained by enhancing the specimen with xylene and examining under phase microscopy.
Seminal fluid contains a high concentration of PAP, therefore the
detection of this enzyme can aid in determining the presence of semen in a specimen.
A more specific method is the detection of seminal glycoprotein p30
Further, information can often be obtained by performing ABO blood
grouping and DNA analysis on the specimen.
47 Semen Analysis 48 Semen Analysis Exercises
1. The major component of seminal fluid :
2. If the first portion of a semen specimen is not collected, the semen analysis will have an abnormal: 3. Failure of laboratory personnel to document the time a semen sample is collected primarily affects the interpretation of semen: 4. A semen specimen delivered to the laboratory in a condom has a normal sperm count and markedly decreased sperm motility. This is indicative of: 5. An increased semen ph may be caused by:
49 Semen Analysis References: Henry’s Clinical Diagnosis and Management by Laboratory Methods 22nd edition 2011 Clinical chemistry: Principles, procedures, correlation. 6th ed. Michael L. Bishop et al. 2010 Urinalysis and body fluids / Susan King Strasinger, 5th ed. 2008 Tietz Text book of clinical chemistry. 6th ed. Carl AB, Edward RA, 2007 District laboratory practice in tropical countries. 2nd ed. Part I. Monica Cheesbrough, 2005 Clinical chemistry: Theory, analysis, correlation 4th ed. Lawrence AK. 2003 Text book of urinalysis and body fluids. Doris LR, Ann EN, 1983 Urinalysis and body fluids: A color text and atlas. Karen MR, Jean JL. 1995
Chiari - Frommel Syndrome - Sexual Dysfunction, Sexual Intercourse Discomfort & Loss of Sexual Desire Related To Dryness in The Vagina Secondary To Gal Actor Rhea
Chiari - Frommel Syndrome - Sexual Dysfunction, Sexual Intercourse Discomfort & Loss of Sexual Desire Related To Dryness in The Vagina Secondary To Gal Actor Rhea
