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Semen Analysis
(based on WHO guidelines 2010)
Constituents of Semen
● Normal semen is an admixture of spermatozoa
suspended in secretions (seminal plasma) from
glandular tissues of male genital system.
● Testes produces spermatozoa and constitutes
5% of the semen volume.
● Vas deferens produces ergothionine
● Epididymis ( maturation/ storage of sperm)
produces:
– Choline - energy source of sperms.
– Alpha glucosidase
– Carnitine
● Seminal vesicle – nutritive fluid containing
fructose, and is secreted during ejaculation.
(50% of semen volume)
● Prostate produces (40% of semen volume)
– Citric acid
– Acid phosphatase
– Proteolytic enzyme
– Zinc
● Bulbourethral glands of Cowper produces
mucous. ( constitutes 5% of semen volume)
● Indications of Semen Analysis
● Investigation of infertility
● Check effectiveness of vasectomy
● Paternity testing
● Rape cases
● Selection of donors for artificial insemination/
assisted reproductive technology.
● Sample collection
– Sample should be collected after 48 hrs of
abstinence. Higher abstinence → decreased
motility. Lesser abstinence → decreased count.
– Collection is done by masturbation.
Not recommended: condom collection, coitus
interruptus. (loss of initial portion of the ejaculate)
– Collection should be done in a clean, wide mouth,
leak proof container.
● Transport
– Should be done within one hour to the laboratory.
– Temperature should be maintained as close to the
body temperature as possible (inside pocket)
● Two specimens should be examined at least 2
to 3 weeks apart.
Examination of Seminal fluid in
Infertility
● Physical examination
– Visual appearance : opaque to grey – white, slightly
yellow after abstinence.
● Inflammation of male accessory organs → yellow color of
semen → pyospermia
● White clear semen → azoospermia
● Brown or red color → hemospermia
– Viscosity
● Assessed by filling a pipette with semen and allowing it to
flow back to the container
● Normal semen fall drop by drop
● If droplet form threads > 2 cm long → increased viscosity
● Normal semen liquefies in 30 min. If liquefaction does not
occur in 60 min → abnormal increase in viscosity. This
decreases sperm motility.
● If sample does not liquefy → treat with plasmin or
chymotrypsin.
● Volume : more than 1.5 ml
– If the sample volume is less than 1 ml spillage or
incomplete collection must be ruled out
– Conditions leading to low semen volume
(hypospermia)
● Disorders of seminal vesicles or prostate
● Retrograde ejaculation
● Congenital absence of prostate or seminal vesicle
● PH : normal >= 7.2
– Seminal vesicle secretion is basic
– Prostatic secretion is acidic
– If pH = 7 with absence of sperm → indicates either
obstruction of ejaculatory duct or absence of vas
deferens.
Microscopic examination
● Motility
– Ability of the sperm to move
– 3 types of motility
● Rapidly progressive – moving fast and forward in a
straight line
● Slowly progressive – crooked, curved, slow forward
movement
● Non progressive – movement of tail only
– Only those sperms with rapid progressive
movement are capable of fertilizing an ovum.
– Method
● A drop of semen is placed on a slide, covered with
coverslip and sealed with petroleum jelly.
● Examination is done under 40x
● Count at least 200 spermatozoa
● Find the percentage of rapidly progressive, slowly
progressive, non progressive and non motile sperm.
● Normal values
– > 32 % progressive motility
– > 40 % progressive + non progressive motility
● Vitality
– Number of live sperms are called viable
– A viable sperm will have intact cell membrane and
will not take up eosin Y
– Method
● 1 drop of semen + 1 drop of eosin – nigrosin
● Wait for 30 sec
● Put a drop on a slide
● Air dry
● Examine under oil immersion and count 200 sperms
● Red sperms not viable; white sperm viable
● Normal viable count > 58%
● Count
– Wait for liquefaction
– Mix 1ml semen with 20 ml diluting fluid(sodium
bicarbonate – formalin)
– Charge Neubauer’s chamber with pateur’s pipette
– Place chamber in humid conditions for 10 – 15 min
– Count in 4 large chambers
– Calculation
count = sperm counted x correction for dil. Fluid x1000
–--------------------------------------------------
No. of squares counted x vol of 1 square
= N x 20 x1000
-------------
4 x 0.1
= N x 50,000
– Normal count > 15 million/ ml
● Morphology
– Drop of seminal fluid on the slide
– Stain with pap/eosin-nigrosin/rose bengal-toludine
blue
– Examine the morphology of at least 200 sperms
– Normal > 4 % of sperm should have normal
morphology.
● Normal morphology of spermatozoa
– Head : consists of nucleus with condensed chromatin
and some nuclear vacuoles.
– Acrosome: anterior 2/3rd of the head shows an
acrosom cap, secrets enzymes that dissolve the cells
of corona radiata and zona pellucida of the ovum
during fertilization.
– Middle piece contains mitochondria → provides
energy.
– The tail used for motility.
Immunological analysis (antisperm antibody
determination )
● Sperm Mar Test
– Direct SMT
● For detection of sperms coated with IgG/IgA
– Indirect SMT
● For detections of antisperm IgG/A antibodies in serum.
● Immunobead test
– Similar to sperm mar test but uses plastic beads
instead of latex particles to detect
antigen/antibodies
● Normal
– <50 % motile spermatozoa with bound particles.
Biochemical Analysis
● Seminal vesicle marker (Fructose)
– 50 mg of resorcinol in 33ml of conc. Hcl then diluted
with 100 ml of Distilled water.
– 0.5 ml of seminal fluid is added
– The mixture is heated → produces red precipitate in
30 seconds
– Presence of red precipitate indicates presence of
Fructose
– Absence of fructose → no seminal vesicle present
● D/t obstructed vas deferens or absent seminal vesicle.
Sperm function test
● Post coital (Sims-Huhner) test
– Principle
● Examination of the quality of cervical mucus post coitus can
give an idea about the quality of cervical mucus and the ability
of the sperm to penetrate it.
● Normally in proliferative phase (estrogen phase), mucus is
watery and sperm can penetrate easily.
● During secretory phase (progesterone phase), mucus is viscus.
● Hence testing mucus is scheduled just before ovulation.
– Method
● Cervical mucus is aspirated 2 – 12 hrs after intercourse.
– Gross examination
● Normal – mucus stretches at least 2 inches, dries in fern
like pattern.
● Abnormal – can not stretch 2 in. No fern like pattern on
drying.
– Microscopic examination
● Normal – more than or equal to 10 motile sperms
● Abnormal – less than 10 motile sperms
– Causes – antisperm antibodies, cervicitis, wrong judgement of
date.
● Cervical mucus penetration test
– Evaluation of the distance traveled by sperm in bovine mucus.
– Fertile sperm travel > 30mm
– Infertile sperm travel <20 mm
● Hamster egg penetration assay
– Hamster egg → enzymatically treated → removal of outer coat
– Incubate with sperm
– Look for number of eggs penetrated ( <15% indicate low fertility ) and
number of sperm penetrating the egg (normal > = 5%)
● Hypoosmotic swelling of flagella
– If sperm is exposed to hypoosmotic solution, sperm
curls up if plasma membrane is abnormal.
– Assessment of functional integrity of plasma
membrane.
● Computer assisted semen analysis
– All above parameters are measured by automated
machines.
Summary of normal values
(WHO 2010)

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Semen analysis

  • 1. Semen Analysis (based on WHO guidelines 2010)
  • 2. Constituents of Semen ● Normal semen is an admixture of spermatozoa suspended in secretions (seminal plasma) from glandular tissues of male genital system.
  • 3. ● Testes produces spermatozoa and constitutes 5% of the semen volume. ● Vas deferens produces ergothionine ● Epididymis ( maturation/ storage of sperm) produces: – Choline - energy source of sperms. – Alpha glucosidase – Carnitine
  • 4. ● Seminal vesicle – nutritive fluid containing fructose, and is secreted during ejaculation. (50% of semen volume) ● Prostate produces (40% of semen volume) – Citric acid – Acid phosphatase – Proteolytic enzyme – Zinc ● Bulbourethral glands of Cowper produces mucous. ( constitutes 5% of semen volume)
  • 5. ● Indications of Semen Analysis ● Investigation of infertility ● Check effectiveness of vasectomy ● Paternity testing ● Rape cases ● Selection of donors for artificial insemination/ assisted reproductive technology.
  • 6. ● Sample collection – Sample should be collected after 48 hrs of abstinence. Higher abstinence → decreased motility. Lesser abstinence → decreased count. – Collection is done by masturbation. Not recommended: condom collection, coitus interruptus. (loss of initial portion of the ejaculate) – Collection should be done in a clean, wide mouth, leak proof container.
  • 7. ● Transport – Should be done within one hour to the laboratory. – Temperature should be maintained as close to the body temperature as possible (inside pocket) ● Two specimens should be examined at least 2 to 3 weeks apart.
  • 8. Examination of Seminal fluid in Infertility ● Physical examination – Visual appearance : opaque to grey – white, slightly yellow after abstinence. ● Inflammation of male accessory organs → yellow color of semen → pyospermia ● White clear semen → azoospermia ● Brown or red color → hemospermia
  • 9. – Viscosity ● Assessed by filling a pipette with semen and allowing it to flow back to the container ● Normal semen fall drop by drop ● If droplet form threads > 2 cm long → increased viscosity ● Normal semen liquefies in 30 min. If liquefaction does not occur in 60 min → abnormal increase in viscosity. This decreases sperm motility. ● If sample does not liquefy → treat with plasmin or chymotrypsin.
  • 10. ● Volume : more than 1.5 ml – If the sample volume is less than 1 ml spillage or incomplete collection must be ruled out – Conditions leading to low semen volume (hypospermia) ● Disorders of seminal vesicles or prostate ● Retrograde ejaculation ● Congenital absence of prostate or seminal vesicle
  • 11. ● PH : normal >= 7.2 – Seminal vesicle secretion is basic – Prostatic secretion is acidic – If pH = 7 with absence of sperm → indicates either obstruction of ejaculatory duct or absence of vas deferens.
  • 12. Microscopic examination ● Motility – Ability of the sperm to move – 3 types of motility ● Rapidly progressive – moving fast and forward in a straight line ● Slowly progressive – crooked, curved, slow forward movement ● Non progressive – movement of tail only
  • 13. – Only those sperms with rapid progressive movement are capable of fertilizing an ovum. – Method ● A drop of semen is placed on a slide, covered with coverslip and sealed with petroleum jelly. ● Examination is done under 40x ● Count at least 200 spermatozoa ● Find the percentage of rapidly progressive, slowly progressive, non progressive and non motile sperm. ● Normal values – > 32 % progressive motility – > 40 % progressive + non progressive motility
  • 14. ● Vitality – Number of live sperms are called viable – A viable sperm will have intact cell membrane and will not take up eosin Y – Method ● 1 drop of semen + 1 drop of eosin – nigrosin ● Wait for 30 sec ● Put a drop on a slide ● Air dry ● Examine under oil immersion and count 200 sperms ● Red sperms not viable; white sperm viable ● Normal viable count > 58%
  • 15. ● Count – Wait for liquefaction – Mix 1ml semen with 20 ml diluting fluid(sodium bicarbonate – formalin) – Charge Neubauer’s chamber with pateur’s pipette – Place chamber in humid conditions for 10 – 15 min – Count in 4 large chambers
  • 16. – Calculation count = sperm counted x correction for dil. Fluid x1000 –-------------------------------------------------- No. of squares counted x vol of 1 square = N x 20 x1000 ------------- 4 x 0.1 = N x 50,000 – Normal count > 15 million/ ml
  • 17. ● Morphology – Drop of seminal fluid on the slide – Stain with pap/eosin-nigrosin/rose bengal-toludine blue – Examine the morphology of at least 200 sperms – Normal > 4 % of sperm should have normal morphology.
  • 18. ● Normal morphology of spermatozoa – Head : consists of nucleus with condensed chromatin and some nuclear vacuoles. – Acrosome: anterior 2/3rd of the head shows an acrosom cap, secrets enzymes that dissolve the cells of corona radiata and zona pellucida of the ovum during fertilization. – Middle piece contains mitochondria → provides energy. – The tail used for motility.
  • 19.
  • 20.
  • 21. Immunological analysis (antisperm antibody determination ) ● Sperm Mar Test – Direct SMT ● For detection of sperms coated with IgG/IgA – Indirect SMT ● For detections of antisperm IgG/A antibodies in serum.
  • 22. ● Immunobead test – Similar to sperm mar test but uses plastic beads instead of latex particles to detect antigen/antibodies ● Normal – <50 % motile spermatozoa with bound particles.
  • 23. Biochemical Analysis ● Seminal vesicle marker (Fructose) – 50 mg of resorcinol in 33ml of conc. Hcl then diluted with 100 ml of Distilled water. – 0.5 ml of seminal fluid is added – The mixture is heated → produces red precipitate in 30 seconds – Presence of red precipitate indicates presence of Fructose – Absence of fructose → no seminal vesicle present ● D/t obstructed vas deferens or absent seminal vesicle.
  • 24. Sperm function test ● Post coital (Sims-Huhner) test – Principle ● Examination of the quality of cervical mucus post coitus can give an idea about the quality of cervical mucus and the ability of the sperm to penetrate it. ● Normally in proliferative phase (estrogen phase), mucus is watery and sperm can penetrate easily. ● During secretory phase (progesterone phase), mucus is viscus. ● Hence testing mucus is scheduled just before ovulation.
  • 25. – Method ● Cervical mucus is aspirated 2 – 12 hrs after intercourse. – Gross examination ● Normal – mucus stretches at least 2 inches, dries in fern like pattern. ● Abnormal – can not stretch 2 in. No fern like pattern on drying. – Microscopic examination ● Normal – more than or equal to 10 motile sperms ● Abnormal – less than 10 motile sperms – Causes – antisperm antibodies, cervicitis, wrong judgement of date.
  • 26. ● Cervical mucus penetration test – Evaluation of the distance traveled by sperm in bovine mucus. – Fertile sperm travel > 30mm – Infertile sperm travel <20 mm ● Hamster egg penetration assay – Hamster egg → enzymatically treated → removal of outer coat – Incubate with sperm – Look for number of eggs penetrated ( <15% indicate low fertility ) and number of sperm penetrating the egg (normal > = 5%)
  • 27. ● Hypoosmotic swelling of flagella – If sperm is exposed to hypoosmotic solution, sperm curls up if plasma membrane is abnormal. – Assessment of functional integrity of plasma membrane. ● Computer assisted semen analysis – All above parameters are measured by automated machines.
  • 28. Summary of normal values (WHO 2010)