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Sperm chromatin integrity has been being recognized as an important factor in male fertility. During normal fertilization, high quality sperm with intact chromatin are selected through natural selection in journey from vagina to fallopian tube. However, using Assisted Reproductive Techniques, particularly ICSI, the natural selection is bypassed. Therefore sperm with DNA breakage have the opportunity to fertilize the egg which may lead to decreased embryo quality and implantation rate. The aim of this study was to evaluate the effects of sperm chromatin integrity on ICSI outcomes. A total of 200 semen samples were collected from couples undergoing ICSI and were analyzed according to WHO criteria. Each sample was evaluated for sperm chromatin integrity using four cytochemical assays and semen processing by swim up method. The ICSI was carried out according to a long-term pituitary down-regulation protocol. The correlation between sperm parameters, sperm chromatin integrity and ICSI outcomes (fertilization rate and embryo quality) was examined. The mean number of oocyte, fertilization rate and cleavage embryos per cycles was 7.5±5.0, 74.06%±25 and 5.4±3.6, respectively. There was not significant correlation between the results of chromatin assays (AO, AB, TB, and CMA3) and fertilization outcomes following ICSI. The fertilization rate was significantly higher for a group with less than 10% chromatin abnormality (p<0.05). Sperm chromatin integrity is essential for successful fertilization, embryo development and normal pregnancy. A protamine deficiency appeared to affect fertilization rate and embryo quality. However, the presence of confounding factors such as selection of spermatozoa according to normal morphology may influence the effect of sperm chromatin status on ICSI outcomes.
The field of Assisted Reproductive Technology (ART) including ICSI, IVF and IUI has been significantly developed in the last two decades and consequently demand for such treatments have dramatically increased. In Europe, the number of ART treatment is more than 270,000 per year (
Among various assisted reproductive techniques, ICSI has become a preferred and widely applied method for helping infertile couples to achieve conception (
Sperm functional assay is considered as the valuable diagnostic tool in evaluation and prediction of male infertility (
A total of 200 semen samples were collected from couples undergoing ICSI at Avicenna Infertility Clinic (AIC), Tehran, Iran. The informed written consent for use of the surplus semen in this research was obtained from the couples in accordance with the Avicenna Research Institute Medical Ethics regulation in research involving the human subjects. The cryopreserved semen samples and also samples with less than 1×106
Briefly, on the day of oocyte aspiration, semen sample was produced on-site by masturbation and allowed to liquefy at 37
The Controlled Ovarian Hyperstimulation (COH) was performed according to the long luteal suppression protocol, using a GnRHa (Superfact, Ferring, Germany) and combination of HMG (Menogon, Ferring, Germany) or recombinant FSH (Gonal-F, Serono, Switzerland). The ovulation was induced when at least three follicles had a diameter of ≥18
The oocytes were assessed for fertilization at 16-18
The method for Acridine Orange staining was the modified protocol previously described (
The air-dried smears were fixed according to AO staining and allowed to dry for a few minutes before staining with 0.05% Toluidine Blue (Merck, Germany) in staining buffer for 10
The air-dried fixed smears were treated for 20
As a positive control, semen samples were treated with hydrogen peroxide 100
The air-dried fixed smears were stained for 7
Fertilization rates were calculated for each cycle as the number of cleavage embryos divided by the number of metaphase Π oocytes. The correlations between the sperm parameters, sperm chromatin assay results, fertilization rate and embryo quality were evaluated by calculating Pearson's correlation coefficient (r). To test the statistical significance of the results, a non-parametric method of the Mann-whitney U test was used. All statistical analyses were carried out using SPSS Version 11.5 (SPSS Inc, USA, IL).
For this study, 200 semen samples were collected. A sample of 28 were excluded from the study due to insufficient volume of semen sample, lack of oocyte retrieval following puncture and due to anomalies and low quality of oocytes. The mean age of male participant was 33.9±6
Summery of semen analysis and sperm chromatin assay results in 172 men undergoing ICSI treatment
| Mean±SD | |
|---|---|
|
|
2.4±1.1 |
|
|
83±59 |
|
|
260±226.8 |
|
|
24.71±9.4 |
|
|
|
|
|
11.18±8.46 |
|
|
21.83±8.9 |
|
|
16.06±6.2 |
|
|
50.9±14.4 |
|
|
|
|
|
26.5±13.0 |
|
|
27.1±13.0 |
|
|
31.4±13.6 |
|
|
36.2±12.9 |
Percentage of sperm with abnormal chromatin
Summary of embryology results in 172 couples undergoing ICSI cycle
| Mean±SD | |
|---|---|
|
|
7.5±5.0 |
|
|
5.4±3.6 |
|
|
3.5±1.0 |
|
|
74.06±25 |
|
|
|
|
|
58.1±33 |
|
|
37±31 |
|
|
4.9±1.4 |
The mean fertilization rate was 74.06±25 and there were no significant correlations between sperm function tests and fertilization rate. However, when chromatin integrity was measured by aniline blue divided in two groups according to a threshold of 10%, the fertilization rate was significantly higher for the group with less than 10% chromatin abnormality (85±22.3 vs. 73.4±25.4) (p < 0.05). However this was not significant for grouping according to thresholds of 20% or 30%. Also, the fertilization rate following ICSI was not influenced by sperm parameters of motility, morphology and concentration (p > 0.05) (
The average percentage of embryo quality (grade A, B, C) is summarized in
Correlation between sperm function test results and embryo quality
| Grade A | Grade B | Grade C | ||||
|---|---|---|---|---|---|---|
|
|
||||||
| Test | r | p-value | r | p-value | r | p-value |
|
|
||||||
|
|
0.05 | NS | -0.06 | NS | -0.006 | NS |
|
|
0. 074 | NS | -0.03 | NS | -0.09 | NS |
|
|
-0. 071 | NS | 0.05 | NS | 0.042 | NS |
|
|
0.207 | 0.017 |
-0.2 | 0.01 |
-0.71 | NS |
p < 0.05
Percentage of sperm with abnormal chromatin, NS= not statistically significant;
In the present study, four different cytohemical staining methods including Toluidine Blue, Aniline Blue, Chromomycin A3 and Acridine Orange assays were applied in order to assess different aspects of sperm DNA integrity (
Our results showed that when the cases were divided in two groups according to chromatin abnormality, fertilization rates were significantly increased in the group with less than 10% abnormal chromatin threshold using Aniline Blue. Such finding may indicate that protamine deficiency has considerable affect on fertilization rate. However in case of grouping by 20% or 30% thresholds of abnormal chromatin, no significant differences were found between the two groups. We also found no significant correlation between other chromatin staining assays and fertilization rate. This was in agreement with Sakass and Zini (
Normal sperm chromatin structure and integrity is essential for the accurate transmission of paternal genetic information to the next generation and also appropriate function of sperm in the fertilization process (
A reason for the current findings of "no significant correlation between fertilization rates and most of the sperm parameters" may be due to the fact that assays for sperm chromatin abnormalities were performed on raw semen samples that contained large numbers of immotile, nonviable or degenerated sperm with abnormal chromatin. However, through pre-ICSI processing techniques (gradient centrifugation, swim up or glass wool, etc.) most abnormal sperms are removed and the resultant processed semen contain motile sperm with normal morphology (
Indeed the aim of pre-ICSI processing techniques is to select the best quality spermatozoa during ICSI and as far as possible to avoid the transfer of the genetic abnormalities to oocyte that is similar to the natural selection during
Another reason that may explain the lack of relationship between sperm parameters and fertilization rate in our study and related studies could be due to the fact that during ICSI procedure, the operator′s attempt to select motile and morphologically normal spermatozoa may affect the ICSI outcomes as a confounding factor. This could be the second level of sperm selection in ICSI procedure substituted by the natural selection in normal pregnancy that may slightly reduce the risk of transfer of genetic abnormalities in ICST.
We also found a significant difference in embryo quality grade A between groups below and above 30% abnormal chromatin using Chromomycin A3 staining. The finding indicates that chromatin abnormality as well as fertilization rate can affect embryo quality. Although the impact of chromatin abnormality remains controversial, there is a wider agreement about its negative affect on embryo development (
In conclusion, considering the importance of sperm chromatin structure in protecting sperm genome, abnormal structures of chromatin could have negative influences in the ART outcomes. The present study indicated that protamine deficiency could affect fertilization rate and embryo quality. Thus improving methods for selecting sperm with intact chromatin is suggested. However, there are confounding factors such as pre-ICSI processing techniques and selecting spermatozoa with normal morphology and motility that may influence the assessment of the affect of sperm chromatin status on ICSI outcome.
Indeed the sperm pre-selection process during ICSI procedure, that is substitute to the natural selection barrier in normal pregnancy, could affect the validity of the studies performed to find the correlation between sperm quality and fertilization outcomes. More precise studies with reduced confounding factors are needed to evaluate the correlation between sperm parameters and ICSI.
The authors would like to thank Dr H. Zeraati for assistance with statistical analyses and S. Behnam Hashemi (MD, MPH) for kindly editing the article.