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SPERM CHROMATIN STRUCTURE ASSAY
SPERM CHROMATIN DISPERSION TEST
SPERM DNA
• Sperm DNA differs from the somatic DNA
• DNA completely occupy nucleus
• 9.9µm^3 -> twice
• Protamine's
• DNA domains loop – Donut shape toroid
• Protamine's and MAR fixed below
• Toroid -> Disulfide bond
• Histones
SPERM CHROMATIN DISPERSION
• Fenandez 2003
• When sperm is treated with an acid solution
prior to the lysis buffer, absence or minimal
halo is produced -> fragmented DNA
• Sperm DNA acid solution depolarized nuclei
lysis solution
Forms halo indicates Absent halo
DNA intact DNA damage
Principle
• When sperms are treated with an acid
solution prior to lysis buffer, the DNA
dispersion halos that are observed in sperm
nuclei with non-fragmented DNA due to
altered nuclear protein
• Which is minimal present or not present at
all in sperm nuclei with fragmented DNA
• Observed in fluorescent microscopy
PREPARATION
• Sperm conc with 5-10 million / ml prepared with PBS
• Mix with 1ml low M.P agarose at 37˚ C
• 50µl -> glass slide coated with 0.65% standard agarose dried at
80˚C put coverslip
• Solidify ( agarose) for 4 min at 4˚C in fridge
• Coverslip is removed
• Horizontally immersed in the tray of freshly prepared acid
denaturation solution (0.08N HCL) for 7 min in dark
• Transfer the slide to tray with neutralizing and lysing solution 1
for 10 min
• Neutralizing and lysing solution 2 incubate for 5 min
• Wash -> Tris – borate EDTA buffer for 2 min
• Dehydrated with 70%, 50%, 100% ethanol baths 2 min each
• Air-dried
• Stained with DAPI for florescence microscopy
DFI
• Sperm nucleoid has *central core * outer
halo
• SDFI = 100 ˣ Fragmented + degraded
Total cells
ADVANTAGE
• Minimal requirement
• Simple
• Cost effective
• Oxidative DNA damage can be determined
by adding 8- oxoguanine DNA probe
The Sperm Chromatin Structure Assay
• 1980s -> DNA fragmentation
• First test
• Evenson
• Detect the damaged sperm DNA and altered protein
in sperm nuclei, view flow cytometry, acridine
orange (AO) stained sperm
• 2 types : SCSA heat and SCSA acid
• SCSA acid is frequently used
• Abnormal protein / DNA complex/ immature
spermatozoa -> AO dye -> high HDS ( high level DNA
stainability)
Principle
• SCSA relies on the fact that abnormally
sperm chromatin has a greater susceptibility
to the physical induction of partial DNA
denaturation in situ
• Extent of DNA denaturation following heat
or acid treatment is determined by
measuring the metachromatic shift from
green fluorescents to red fluorescents
• By flow cytometry
• AO binds to DNA helix as an intercalate and
emits green fluorescence when bounded to
intact ds DNA
• Red fluorescence when bound to fragmented
DNA
Preparation
• Stained sample -> flow cytometry -> fluidics system
transport spermatozoa in a stream to the laser beam
of interrogation
• Optics system illuminates the particle and directs the
resulting light signals to the appropriate detector
• Equipment convers light signals to electronic system
-> processes by dedicated software
• % DFI = DNA stainability with red fluorescence
intensity / total red + green florescence
• Left panel -> Total DNA stainability v/s DFI
This reorients data into vertical / horizontal
pattern of dots
• Right panel -> frequency histogram of DFI
 Non – detectable DNA fragmentation
 Moderate level DNA fragmentation
 High level DNA fragmentation
• Total 5000 sperms are recorded on flow
cytometer
Advantages
• Abnormal sperm -> lack of protamine's
• Most precise
• Non-biased flow cytometer machine
• Repeatability
• cut-off point (25% DFI) to differentiate
between fertile and infertile samples
• successful assay ->ART -> fertilization and
implantation
Reference
• Assessment of sperm deoxyribose nucleic acid fragmentation
using sperm chromatin dispersion assay
• Textbook of assisted reproductive techniques vol1
• Clinical application of Sperm Chromatin Structure Assay in
diagnosis and treatment of infertility
• The Sperm Chromatin Structure Assay (SCSA®) and other sperm
DNA fragmentation tests for evaluation of sperm nuclear DNA
integrity as related to fertility
• Sperm chromatin structure assay (SCSA ® ) Article in Methods in
Molecular Biology
• Sperm chromatin assessment Ashok Agarwal, Tamer M Said
• The Sperm Chromatin Dispersion Test: A Simple Method for the
Determination of Sperm DNA Fragmentation
• Sperm chromatin dispersion test in the assessment of DNA
fragmentation and aneuploidy in human spermatozoa
Sperm Chromatin Structure Assay

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Sperm Chromatin Structure Assay

  • 1. SPERM CHROMATIN STRUCTURE ASSAY SPERM CHROMATIN DISPERSION TEST
  • 2. SPERM DNA • Sperm DNA differs from the somatic DNA • DNA completely occupy nucleus • 9.9µm^3 -> twice • Protamine's • DNA domains loop – Donut shape toroid • Protamine's and MAR fixed below • Toroid -> Disulfide bond • Histones
  • 3.
  • 4.
  • 5.
  • 6. SPERM CHROMATIN DISPERSION • Fenandez 2003 • When sperm is treated with an acid solution prior to the lysis buffer, absence or minimal halo is produced -> fragmented DNA • Sperm DNA acid solution depolarized nuclei lysis solution Forms halo indicates Absent halo DNA intact DNA damage
  • 7. Principle • When sperms are treated with an acid solution prior to lysis buffer, the DNA dispersion halos that are observed in sperm nuclei with non-fragmented DNA due to altered nuclear protein • Which is minimal present or not present at all in sperm nuclei with fragmented DNA • Observed in fluorescent microscopy
  • 8.
  • 9. PREPARATION • Sperm conc with 5-10 million / ml prepared with PBS • Mix with 1ml low M.P agarose at 37˚ C • 50µl -> glass slide coated with 0.65% standard agarose dried at 80˚C put coverslip • Solidify ( agarose) for 4 min at 4˚C in fridge • Coverslip is removed • Horizontally immersed in the tray of freshly prepared acid denaturation solution (0.08N HCL) for 7 min in dark • Transfer the slide to tray with neutralizing and lysing solution 1 for 10 min • Neutralizing and lysing solution 2 incubate for 5 min • Wash -> Tris – borate EDTA buffer for 2 min • Dehydrated with 70%, 50%, 100% ethanol baths 2 min each • Air-dried • Stained with DAPI for florescence microscopy
  • 10.
  • 11. DFI • Sperm nucleoid has *central core * outer halo • SDFI = 100 ˣ Fragmented + degraded Total cells
  • 12. ADVANTAGE • Minimal requirement • Simple • Cost effective • Oxidative DNA damage can be determined by adding 8- oxoguanine DNA probe
  • 13. The Sperm Chromatin Structure Assay • 1980s -> DNA fragmentation • First test • Evenson • Detect the damaged sperm DNA and altered protein in sperm nuclei, view flow cytometry, acridine orange (AO) stained sperm • 2 types : SCSA heat and SCSA acid • SCSA acid is frequently used • Abnormal protein / DNA complex/ immature spermatozoa -> AO dye -> high HDS ( high level DNA stainability)
  • 14. Principle • SCSA relies on the fact that abnormally sperm chromatin has a greater susceptibility to the physical induction of partial DNA denaturation in situ • Extent of DNA denaturation following heat or acid treatment is determined by measuring the metachromatic shift from green fluorescents to red fluorescents • By flow cytometry
  • 15. • AO binds to DNA helix as an intercalate and emits green fluorescence when bounded to intact ds DNA • Red fluorescence when bound to fragmented DNA
  • 16.
  • 18.
  • 19. • Stained sample -> flow cytometry -> fluidics system transport spermatozoa in a stream to the laser beam of interrogation • Optics system illuminates the particle and directs the resulting light signals to the appropriate detector • Equipment convers light signals to electronic system -> processes by dedicated software
  • 20.
  • 21.
  • 22.
  • 23. • % DFI = DNA stainability with red fluorescence intensity / total red + green florescence • Left panel -> Total DNA stainability v/s DFI This reorients data into vertical / horizontal pattern of dots • Right panel -> frequency histogram of DFI  Non – detectable DNA fragmentation  Moderate level DNA fragmentation  High level DNA fragmentation • Total 5000 sperms are recorded on flow cytometer
  • 24. Advantages • Abnormal sperm -> lack of protamine's • Most precise • Non-biased flow cytometer machine • Repeatability • cut-off point (25% DFI) to differentiate between fertile and infertile samples • successful assay ->ART -> fertilization and implantation
  • 25. Reference • Assessment of sperm deoxyribose nucleic acid fragmentation using sperm chromatin dispersion assay • Textbook of assisted reproductive techniques vol1 • Clinical application of Sperm Chromatin Structure Assay in diagnosis and treatment of infertility • The Sperm Chromatin Structure Assay (SCSA®) and other sperm DNA fragmentation tests for evaluation of sperm nuclear DNA integrity as related to fertility • Sperm chromatin structure assay (SCSA ® ) Article in Methods in Molecular Biology • Sperm chromatin assessment Ashok Agarwal, Tamer M Said • The Sperm Chromatin Dispersion Test: A Simple Method for the Determination of Sperm DNA Fragmentation • Sperm chromatin dispersion test in the assessment of DNA fragmentation and aneuploidy in human spermatozoa