Impact of freezing/thawing technique on sperm DNA integrity in HIV-1 patients

Frainais, Christophe; Vialard, François; Rougier, Nathalie; Aegerther, Philippe; Damond, Florence; Ayel, J.-P.; Yazbeck, Chadi; Hazout, A.; Selva, J.

doi:10.1007/s10815-010-9417-4

Cited by 15 publications

(12 citation statements)

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“…Cryopreservation was performed as previously described elsewhere (Frainais et al, 2010). Briefly, the sperm suspension was frozen by a trained operator after drop‐wise dilution with a cryoprotectant (Spermfreeze, 15% glycerol in HEPES buffer; Fertipro NV).…”

Section: Methodsmentioning

confidence: 99%

“…Cryopreservation was found to induce chromatin decondensation (as evaluated by aniline blue staining; Hammadeh et al, 1999; Fortunato et al, 2012), or DNA denaturation (as evaluated by an acridine orange test; Spanò et al, 1999; Gandini et al, 2006; Dejarkom and Kunathikom, 2007), whereas another group failed to see negative effects of cryopreservation on chromatin stability when using 1% sodium dodecyl sulfate + 6 mM EDTA (Huret, 1984). More recently, cryopreservation was shown to increase sperm DNA fragmentation (Donnelly et al, 2001; De Paula et al, 2006; Frainais et al, 2010; Zribi et al, 2010; Gosálvez et al, 2011). However, other studies have not evidenced DNA damage after sperm cryopreservation (Duru et al, 2001; Isachenko et al, 2004).…”

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confidence: 99%

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Cryopreservation of Human Spermatozoa Decreases the Number of Motile Normal Spermatozoa, Induces Nuclear Vacuolization and Chromatin Decondensation

Boitrelle¹,

Albert²,

Theillac³

et al. 2012

Journal of Andrology

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Even though cryopreservation of human spermatozoa is known to alter sperm motility and viability, it may also induce nuclear damages. The present study set out to determine whether or not cryopreservation alters motile sperm morphology under high magnification and/or is associated with chromatin decondensation. For 25 infertile men, we used high-magnification microscopy to determine the proportions of various types of motile spermatozoa before and after freezing-thawing: morphometrically normal spermatozoa with no vacuole (grade I), #2 small vacuoles (grade II), at least 1 large vacuole or .2 small vacuoles (grade III), and morphometrically abnormal spermatozoa (grade IV). The spermatozoa's chromatin condensation and viability were also assessed before and after freezing-thawing. Cryopreservation induced sperm nuclear vacuolization. It decreased the proportion of grade I + II spermatozoa (P , .001). It induced a decrease in the sperm viability rate (P , .001) and increased the proportion of sperm with noncondensed chromatin (P , .001). The latter parameter was strongly correlated with sperm viability (r 5 0.71; P , .001). However, even motile sperm presented a failure of chromatin condensation after freezingthawing, because the proportion of sperm with noncondensed chromatin was correlated with high-magnification morphology (r 5 20.49 and 0.49 for the proportions of grade I + II and grades III + IV, respectively; P , .001). Cryopreservation alters the organelle morphology of motile human spermatozoa and induces sperm chromatin decondensation. High-magnification microscopy may be useful for evaluating frozen-thawed spermatozoa before use in assisted reproductive technology procedures (such as intrauterine insemination, in vitro fertilization, and intracytoplasmic sperm injection) and for performing research on cryopreservation methods. If frozen-thawed sperm is to be used for intracytoplasmic sperm injection, morphological selection under high magnification may be of particular value.

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Section: Methodsmentioning

confidence: 99%

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confidence: 99%

Cryopreservation of Human Spermatozoa Decreases the Number of Motile Normal Spermatozoa, Induces Nuclear Vacuolization and Chromatin Decondensation

Boitrelle¹,

Albert²,

Theillac³

et al. 2012

Journal of Andrology

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“…Liquefied, fresh semen samples were evaluated according to the WHO guidelines [34] and prepared on a two-layer, discontinuous concentration gradient (PureSperm 100, Nidacon, Sweden), as described previously [15]. In a glass-bottomed dish (the WillCo-dish from WillCo Wells BV, The Netherlands), 5-10 μl of the sperm fraction obtained after density gradient selection were diluted into a 4 μl microdroplet of 10 % polyvinylpyrrolidone in flushing medium (FertiPro N.V., Belgium).…”

Section: Semen Preparation and Parameters For Whole Spermmentioning

confidence: 99%

High-magnification sperm selection does not decrease the aneuploidy rate in patients who are heterozygous for reciprocal translocations

Chelli

Ferfouri

Boitrelle

et al. 2013

J Assist Reprod Genet

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Problem This study sought to evaluate the value of motile sperm organelle morphology examination (MSOME) for selecting euploid spermatozoa in six patients who were heterozygous for a reciprocal translocation. Method of study We used sperm fluorescence in situ hybridization (FISH) to screen for aneuploidy of the chromosomes involved in the translocations and a putative interchromosomal effect (ICE) for chromosomes 18, X and Y. This procedure was performed on (i) whole sperm (i.e. no selection) and on normal spermatozoa selected (ii) at a magnification typically used for intracytoplasmic sperm injection (ICSI), referred to as "ICSIlike", and (iii) with MSOME. Results The balanced translocation rates did not differ significantly (p=0.81) when comparing whole sperm (57.2 %) with spermatozoa after ICSI-like selection (56.3 %) or after MSOME (53.7 %). Similarly, the aneuploidy rates for ICEs did not differ significantly (p=0.14) when comparing whole sperm (1.9 %), ICSI-selected spermatozoa (3.4 %) and MSOME-selected spermatozoa (1.0 %). Conclusion For patients who are heterozygous for reciprocal translocations, MSOME does not improve the selection of euploid spermatozoa.

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“…Next, slides were washed three times in PBS and analysed after counterstaining with DAPI. Spermatozoa with DNA fragmentation fluoresced blue and green, as previously described (Frainais et al ., ). One thousand spermatozoa were counted.…”

Section: Methodsmentioning

confidence: 97%

Sperm FISH analysis of a 44,X,der(Y),t(Y;15)(q12;q10)pat,rob(13;14)(q10;q10)mat complex chromosome rearrangement

et al. 2013

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Complex chromosome rearrangements (CCR) with two independent chromosome rearrangements are rare. Although CCRs lead to high unbalanced gamete rates, data on meiotic segregation in this context are scarce. A male patient was referred to our clinic as part of a family screening programme prompted by the observation of a 44,X,der(Y),t(Y;15)(q12;q10)pat,rob(13;14)(q10;q10)mat karyotype in his brother. Karyotyping identified the same CCR. Sperm FISH (with locus-specific probes for the segments involved in the translocations and nine chromosomes not involved in both rearrangements) was used to investigate the rearrangements meiotic segregation products and establish whether or not an inter-chromosomal effect was present. Sperm nuclear DNA fragmentation was also evaluated. For rob(13;14) and der(Y), the proportions of unbalanced products were, respectively, 26.4% and 60.6%. Overall, 70.3% of the meiotic segregation products were unbalanced. No evidence of an inter-chromosomal effect was found, and the sperm nuclear DNA fragmentation rate was similar to our laboratory's normal cut-off value. In view of previously published sperm FISH analyses of Robertsonian translocations (and even though the mechanism is still unknown), we hypothesise that cosegregation of der(Y) and rob(13;14) could modify rob(13;14) meiotic segregation.

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Impact of freezing/thawing technique on sperm DNA integrity in HIV-1 patients

Cited by 15 publications

References 50 publications

Cryopreservation of Human Spermatozoa Decreases the Number of Motile Normal Spermatozoa, Induces Nuclear Vacuolization and Chromatin Decondensation

Cryopreservation of Human Spermatozoa Decreases the Number of Motile Normal Spermatozoa, Induces Nuclear Vacuolization and Chromatin Decondensation

High-magnification sperm selection does not decrease the aneuploidy rate in patients who are heterozygous for reciprocal translocations

Sperm FISH analysis of a 44,X,der(Y),t(Y;15)(q12;q10)pat,rob(13;14)(q10;q10)mat complex chromosome rearrangement

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