Preparation and incubation conditions affect the DNA integrity of ejaculated human spermatozoa

Matsuura, Rieko; Takeuchi, Takumi; Yoshida, Atsumi

doi:10.1038/aja.2010.46

Cited by 71 publications

(45 citation statements)

References 32 publications

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“…performed using a small number of sperm, it takes a much longer time until sperm injection, causing the accumulation of reactive oxygen species [3,4]. Such changes in culture conditions have been shown to be involved in the lipid peroxidation of cell membranes, nuclear DNA fragmentation, and delay of embryo development [5][6][7][8]. Several groups have reported the cryopreservation of a small number of sperm using devices for embryo vitrification [9,10] by embedding them into an alginate gel [11] and by injecting them into an empty zona pellucida (ZP) [12][13][14].…”

Section: Introductionmentioning

confidence: 99%

Cryopreservation of a small number of human sperm using enzymatically fabricated, hollow hyaluronan microcapsules handled by conventional ICSI procedures

Tomita

Sakai

Khanmohammadi

et al. 2016

J Assist Reprod Genet

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Purpose We investigated whether enzymatically fabricated hyaluronan (HA) microcapsules were feasible for use in the cryopreservation of a small number of sperm. Methods HA microcapsules were fabricated using a system of water-immiscible fluid under laminar flow. Three sperm were injected into a hollow HA microcapsule using a micromanipulator. Capsules containing injected sperm were incubated in a freezing medium composed of sucrose as the cryoprotectant and then placed in a Cryotop® device and plunged into liquid nitrogen. After thawing, the capsule was degraded by hyaluronidase, and the recovery rate of sperm and their motility were investigated. Results The HA microcapsule measuring 200 μm in diameter and with a 30-μm thick membrane was handled using a conventional intracytoplasmic sperm injection (ICSI) system, and the procedure involved the injection of sperm into the capsule. The HA microcapsules containing sperm were cryopreserved in a Cryotop® device and decomposed by the addition of hyaluronidase. The recovery rate of sperm after cryopreservation and degradation of HA microcapsules was sufficient for use in clinical practice (90 %). Conclusions Hollow HA microcapsules can be used for the cryopreservation of a small number of sperm without producing adverse effects on sperm quality.

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Section: Introductionmentioning

confidence: 99%

Cryopreservation of a small number of human sperm using enzymatically fabricated, hollow hyaluronan microcapsules handled by conventional ICSI procedures

Tomita

Sakai

Khanmohammadi

et al. 2016

J Assist Reprod Genet

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“…It is well known that the testis temperature is approximately 2-3°C below body temperature (Elder and Dale, 2011), as this is required for the production and maintenance of viable spermatozoa (Appell et al, 1977;Setchell, 1998). Despite the numerous articles published on the harmful effects of long-term in-vitro sperm incubation at body temperature, it is still current practice in most IVF laboratories to store prepared sperm samples at this unfavourable temperature prior to their use in assisted reproduction treatment (Matsuura et al, 2010).…”

Section: Introductionmentioning

confidence: 99%

“…The quality of the sperm sample is influenced by various laboratory factors, including: (i) use of different sperm preparation techniques (Boomsma et al, 2007;Chen and Bongso, 1999;Marchesi et al, 2010); (ii) temperature during sperm preparation (Franken et al, 2011;Otsuki et al, 2008); (iii) time interval from sperm preparation to IUI (Yavas and Selub, 2004); and (iv) temperature during long-term in-vitro incubation of prepared sperm samples (Aitken et al, 1996;Makler et al, 1981;Matsuura et al, 2010;Petrella et al, 2003). It is well known that the testis temperature is approximately 2-3°C below body temperature (Elder and Dale, 2011), as this is required for the production and maintenance of viable spermatozoa (Appell et al, 1977;Setchell, 1998).…”

Section: Introductionmentioning

confidence: 99%

Influence of temperature and sperm preparation on the quality of spermatozoa

Thijssen

Klerkx

Huyser

et al. 2014

Reproductive BioMedicine Online

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.be (A Thijssen).Annelies Thijssen graduated in July 2012 with a Masters in biomedical sciences -clinical molecular sciences from the Transnational University Limburg, Diepenbeek, Belgium. She finished her master thesis on 'Methods for optimal sperm selection and preservation in the IVF laboratory' at the Genk Institute for Fertility Technology of the Ziekenhuis Oost-Limburg, Genk, Belgium. In September 2012, she started a PhD project 'Sperm banking in Belgium: medical, ethical and economical aspects', a collaboration between Hasselt University and the Ziekenhuis Oost-Limburg with Willem Ombelet as promoter.Abstract This study investigated the effects of long-term (24 h) in-vitro sperm incubation at room temperature (RT; 23°C) versus testis temperature (35°C) on various sperm-quality parameters. Semen samples (n = 41) were prepared both by density-gradient centrifugation (DGC) and the swim-up technique in order to compare the influence of sperm preparation on sperm quality after incubation. Progressive motility and morphology were significantly higher after incubation at RT compared with 35°C( P < 0.001 and P < 0.01, respectively). The proportions of acrosome-reacted, apoptotic and dead spermatozoa were significantly lower in samples incubated for 24 h at RT compared with 35°C( P < 0.001, P = 0.01 and P < 0.001, respectively). The number of motile, morphologically normal, non-acrosome-reacted and nonapoptotic spermatozoa recovered after sperm preparation was significantly higher in DGC compared with swim-up samples (P < 0.001). However, spermatozoa prepared by swim-up showed better survival after incubation compared with DGC-prepared spermatozoa, especially when incubated at 35°C. In conclusion, this study indicates a significantly better and longer preservation of sperm quality when incubation is performed at RT. These findings may convince laboratories to change the routinely used sperm storage conditions in order to maximize the quality of the prepared sperm sample.

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“…One of the most commonly reported is sperm processing, especially centrifugation and incubation (Bungum et al 2008;Koderle et al 2009;Matsuura et al 2010). Another potential factor is the use of different types of extenders (Shahiduzzaman and Linde-Forsberg 2007;Fernandez-Santos et al 2009;Morrell et al 2009).…”

mentioning

confidence: 99%

DNA integrity in fresh, chilled and frozen-thawed canine spermatozoa

Prinosilova¹,

Rybar²,

Zajicova³

et al. 2012

Vet. Med. - Czech

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Sperm chromatin status in fresh dog semen and the effect of long-term storage of chilled and frozen dog semen on sperm chromatin integrity was assessed by the sperm chromatin structure assay (SCSA). In the first experiment, the chromatin integrity of fresh semen from 60 dogs with different historiy of fertility was compared with other sperm parameters (total sperm count, sperm motility, viability, acrosomal integrity and sperm morphology). Except for 15 dogs that had never mated before, all were used in breeding as semen donors. Thirty-three of them were successful breeding males while in 12 repeated fertility problems were noted. Ejaculates were assigned to groups with good and poor quality, based on determined sperm motility and percentage of morphologically normal sperm. In the second experiment, chromatin status was measured in fresh and chilled spermatozoa (on day 0, 2, 4, 6, 8 and 10 of storage). Finally, in the third experiment, the chromatin status was measured in fresh and cryopreserved spermatozoa. Evaluating fresh dog semen, we observed that DNA fragmentation index (DFI) and percentage of cells with high DNA stainability (HDS) negatively correlated with total sperm count, percentage of total and progressively motile spermatozoa, sperm viability and percentage of morphologically normal spermatozoa, even with rather low correlation indices. Lower chromatin integrity was found in the group of dog ejaculates showing poor quality in comparison with the group of good quality ejaculates. All dogs with repeated fertility problems were classed in the group showing poor quality, and even though their DFI was significantly higher than the DFI of successful breeding males, the highest DFI we obtained was only just below 9%. We can assume that the chromatin damage level in any of the evaluated dogs was not high enough to have a significant effect on their fertility. Concerning the potential cause of reduced male fertility, the assessment of chromatin integrity in fresh dog ejaculates failed to add any additional information to the results obtained by other techniques of semen analysis. Thus, the current study indicates that neither 10-day preservation of canine sperm chilled in commercial extenders nor long-term cryopreservation in extenders recommended for canine sperm preservation produce adverse effects on sperm chromatin integrity.

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Preparation and incubation conditions affect the DNA integrity of ejaculated human spermatozoa

Cited by 71 publications

References 32 publications

Cryopreservation of a small number of human sperm using enzymatically fabricated, hollow hyaluronan microcapsules handled by conventional ICSI procedures

Cryopreservation of a small number of human sperm using enzymatically fabricated, hollow hyaluronan microcapsules handled by conventional ICSI procedures

Influence of temperature and sperm preparation on the quality of spermatozoa

DNA integrity in fresh, chilled and frozen-thawed canine spermatozoa

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