Abstract
OBJECTIVE: In this study, we evaluated whether the hypo-osmotic swelling test (HOST) can be used as a vital marker in combination with peanut agglutinin (PNA) - labeling in fresh and cryopreserved spermatozoa. MATERIALS AND METHODS: Human sperm populations were exposed to a hypo-osmotic medium for 60 minutes, and then incubated in a 1 µg/mL solution of the fluorescent dye Hoescht 33258 (H33258) for 10 minutes. Excess stain was removed by washing in phosphate-buffered saline (PBS) solution, and the pellet was resuspended in 100 µL of culture medium. Twenty microliters of this solution were subsequently smeared on a microscope slide, and fixed in ice-cold methanol to permeabilize the sperm membranes. The fixed smears were finally incubated in a 40-µg/mL FITC-PNA solution for 20 minutes. Simultaneous assessment of acrosome and viability scores was done in a fluorescent microscope equipped with appropriate filters and phase contrast illumination. The same slide was examined for FITC-PNA labeling, tail swelling, and for Hoechst-33258 staining by interchanging the filters and phase contrast optics. RESULTS: In fresh specimens, HOST was found to provide viability assessments comparable to those obtained using the H33258 method (r = 0.95). However, the results of HOST and H33258 were not correlated in cryopreserved specimens (r = 0.22). There was no alteration of PNA-labeling due to the HOST or H33258. CONCLUSIONS: FITC-PNA labeling in conjunction with the visualization of the morphological change induced by exposure to hypo-osmotic solution provides a simple but effective method for establishing the state of acrosomal membrane and viability in fresh human spermatozoa, but this technique is not reliable for cryopreserved ones.
acrosome; sperm; cryopreservation; Fitc pna
CLINICAL UROLOGY
Evaluation of acrosomal status and sperm viability in fresh and cryopreserved specimens by the use of fluorescent peanut agglutinin lectin in conjunction with hypoosmotic swelling test
Sandro C. Esteves; Rakesh K. Sharma; Anthony J. Thomas Jr; Ashok Agarwal
Androfert, Center for Male Infertility, Campinas, Sao Paulo, Brazil, and Reproductive Research Center, Glickman Urological and Kidney Institute, Cleveland Clinic, Cleveland, Ohio, USA
Correspondence Correspondence to Dr. Sandro C. Esteves Androfert Av. Dr. Heitor Penteado, 1464 Campinas, SP, 13075460, Brazil Fax: + 55 19 32946992 Email: s.esteves@androfert.com.br
ABSTRACT
OBJECTIVE: In this study, we evaluated whether the hypoosmotic swelling test (HOST) can be used as a vital marker in combination with peanut agglutinin (PNA) labeling in fresh and cryopreserved spermatozoa.
MATERIALS AND METHODS: Human sperm populations were exposed to a hypoosmotic medium for 60 minutes, and then incubated in a 1 µg/mL solution of the fluorescent dye Hoescht 33258 (H33258) for 10 minutes. Excess stain was removed by washing in phosphatebuffered saline (PBS) solution, and the pellet was resuspended in 100 µL of culture medium. Twenty microliters of this solution were subsequently smeared on a microscope slide, and fixed in icecold methanol to permeabilize the sperm membranes. The fixed smears were finally incubated in a 40µg/mL FITCPNA solution for 20 minutes. Simultaneous assessment of acrosome and viability scores was done in a fluorescent microscope equipped with appropriate filters and phase contrast illumination. The same slide was examined for FITCPNA labeling, tail swelling, and for Hoechst33258 staining by interchanging the filters and phase contrast optics.
RESULTS: In fresh specimens, HOST was found to provide viability assessments comparable to those obtained using the H33258 method (r = 0.95). However, the results of HOST and H33258 were not correlated in cryopreserved specimens (r = 0.22). There was no alteration of PNAlabeling due to the HOST or H33258.
CONCLUSIONS: FITCPNA labeling in conjunction with the visualization of the morphological change induced by exposure to hypoosmotic solution provides a simple but effective method for establishing the state of acrosomal membrane and viability in fresh human spermatozoa, but this technique is not reliable for cryopreserved ones.
Key words: acrosome; sperm; cryopreservation; Fitc pna
INTRODUCTION
Specialized sperm function tests are better predictors of fertilizing potential than traditional semen parameters assessed by standard semen analysis (16). Several functional tests, such as acrosome reaction, hemizona binding assay, sperm morphology, creatine kinase have been proposed to explore sperm fertilization ability and to predict the rate of in vitro fertilization (IVF) (1,3,5,7). The acrosome reaction test (AR) is a stable parameter of sperm function (8,9) which is useful not only to predict fertilization success, but also as a tool in andrology for research purposes, such as male contraception (10) and gonadotoxic effects of food and drugs (11). The test is based on sperm physiology, and involves capacitation and acrosome reaction. Capacitation prepares the sperm to undergo the acrosome reaction with the accompanying release of lytic enzymes and exposure of membrane receptors, which are required for sperm penetration through the zona pellucida and for fusion with the oolema (12).
Several techniques have been proposed to differentiate acrosomeintact from acrosomereacted spermatozoa, including cytochemical staining techniques (13,14), indirect immunofluorescence using monoclonal antibodies (15), labeling with fluoresceinated lectins (16,17) and phasecontrast microscopy to examine partial head decondensation (18). There are significant problems associated to the use of the acrosome reaction on endpoint in the evaluation of human sperm function (14,15,17). One of the most important involving the diagnostic technique is the difficulty in differentiating between pathologic acrosomal loss, secondary to a reduction in cell viability, and a true acrosome loss. Although this problem may be overcome by using a DNAsensitive fluorochromes to monitor viability, such as Hoechst33258, the technique is laborintensive and requires dual filter set to allow simultaneous assessment of the acrosome status and viability (16,19). The differentiation between pathological and true acrosomal loss is particularly important when assessing the acrosome status of cryothawed spermatozoa, because cryopreservation directly damages sperm membrane, resulting in loss of membrane permeability and subsequent cell death (20), as well as in specimens with absence or limited number of motile sperm forms.
The purpose of this study was to evaluate whether the hypoosmotic swelling test (HOST) can be used as a marker of viability in combination with fluoresceine isothiocyanateconjugated peanut agglutinin to monitor the acrosomal status in fresh and cryopreserved spermatozoa.
MATERIALS AND METHODS
Test yolkbuffer freezing medium and sperm washing media (HEPESmodified BiggersWhittenWhittingam) were purchased from Irvine Scientific (Santa Ana, CA). Hoechst 33258 (bisbenzimide), fluoresceine isothiocyanateconjugated peanut agglutinin (FITCPNA), eosin and nigrosin were obtained from Sigma Chemical Company (St. Louis, MO). Hypoosmotic swelling solution was prepared by mixing 7.35 g sodium citrate and 13.51 g fructose in 1 liter of distilled water (21). Hoechst 33258 was prepared as a 1000X stock solution by dissolving 1 mg H33258 in 1 mL Dulbecoo's phosphatebuffered saline. The stock was frozen at 20ºC in 10 mL aliquots in small foilcovered Eppendorf tubes to protect it from light.
Semen samples were obtained from 11 normal healthy volunteer individuals with proven fertility and age ranging from 21 to 35 years old (median 24). Subjects were asked to abstain from ejaculation for at least 48 hours and semen was collected by masturbation into sterile specimen cups. The ejaculate was allowed to liquefy for 30 minutes at 37ºC and examined within 1 hour of collection to determine semen characteristics according to World Health Organization criteria (22). A computer semenanalysis of each specimen was performed on a computerassisted motion analyzer (Motion Analysis; CellTrak, model VP 110, Santa Rosa, CA) to assess concentration and motility. Subjects included in this study were selected according to their basic sperm parameters, as follows: volume > 2.0 mL, concentration > 20 X 106/mL and motility > 50%.
Cryopreservation procedure After initial analysis, each specimen was divided into two aliquots of identical volumes. The first aliquot was cryopreserved while the second aliquot underwent acrosomal and viability assessments. TEST yolkbuffer with glycerol was used as a freezing agent for cryopreservation. Briefly, an aliquot of the freezing medium equal to 25% of the original specimen volume was then added to the specimen. The specimen was gently mixed for 5 minutes using HemaTek aliquot mixer (Miles, Elkhart, Ind.). This was repeated until an equal volume of freezing medium had been added to the ejaculate. The specimen was then equally divided into vials for longterm cryopreservation. Cryovials were placed in the freezer at 20ºC for 8 minutes and thereafter in liquid nitrogen vapor at 100ºC for 2 hours. The vials were then transferred to liquid nitrogen at 196ºC for longterm storage. After at least 2 days in liquid nitrogen, the vials were thawed at 37ºC for 20 minutes, washed twice to remove the cryomedia and reconstituted in modifiedBWW with 5% albumin. After thawing, acrosomal and viability assessments were performed on cryopreserved specimens.
Simultaneous assessment of acrosomal status and viability The protocol developed for assessing the acrosome status involved the use of a detection reagent targeting the acrosomal region of the sperm head (fluorescein isothiocyanateconjugated peanut agglutinin FITCPNA), in conjunction with both the hypoosmotic swelling test (HOST) and the supravital staining Hoechst 33258 to monitor sperm viability. For this assay, 100 mL of the sperm specimens were added to 1 mL of hypoosmotic solution and incubated for 1 hour at 37ºC. At the end of this period, the spermatozoa were pelleted by centrifugation at 1000 rpm for 5 minutes and resuspended in 2 mg/mL Hoechst33258 solution. The sperm suspensions were incubated for 10 minutes in the dark. Spermatozoa were then washed in phosphatebuffered saline (PBS) solution by centrifugation at 1200 rpm for 5 minutes to remove excess stain, and the pellet was resuspended in 100 mL of BWW. Twenty microliters of this solution were subsequently smeared on a microscope slide and allowed to dry. At least three slides of each sample were prepared, in case of problems with labeling or scoring. The slides were then immersed in icecold methanol for 30 seconds to permeabilize the sperm membranes and allowed to air dry. The fixed smears were immersed in a 40µg/mL FITCPNA solution, incubated at room temperature for 20 minutes in foilcovered Coplin jar, and washed gently in PBS to remove the excess label. Scoring was completed within 48 hours of staining.
A Leitz Orthoplan microscope (Leitz, Germany) equipped with phase contrast and fluorescence epiillumination module was used to examine the slides at 1000X magnification in the presence of an antiquenching agent (Cargille immersion oil, type DF, Fisher Scientific, Pittsburgh, PA) to minimize the loss of fluorescence. The same spermatozoon was first examined for tail swelling using phase contrast with halogen illumination (Figure1). Then, the illumination was changed from halogen to mercury ultraviolet epiillumination source for assessing FITCPNA (Figure2) and Hoechst33258 labeling (Figure3). Filter cube I.2 was used for FITCPNA, which fluoresces "applegreen" and cube A.2 for Hoechst33258, which fluoresces a bright medium blue. Examination of the same spermatozoon for FITCPNA labeling and for Hoechst33258 staining was performed by interchanging the two filters. A total of 200 hundred spermatozoa per sample were scored.
Categorization of sperm tail response to hypoosmotic solution and staining patterns Spermatozoa were classified as osmotically competent if tail swelling was observed after exposure to the hypoosmotic solution (Figure1). In contrary, spermatozoa were classified as osmotically incompetent if straight tail was observed. Percentage swelling induced by the cryopreservation process was determined in each specimen after thawing and subtracted from the hypoosmotic swelling test results.
Hoechst33258 stains the nuclei of damaged cells (dead spermatozoa), which show a bright bluewhite fluorescence and is excluded from viable cells (live spermatozoa), which show a pale blue fluorescence. Viability staining on Hoechst33258 was classified as follows. In viable spermatozoa, the sperm head showed a paleblue fluorescence, and in dead spermatozoa, the sperm head showed a bright bluewhite fluorescence (Figure3) (17).
FITCPNA binds specifically to the outer acrosomal membrane. Acrosome staining on FITCPNA labeling was classified as follows. In an intact acrosome, the acrosomal region of the sperm head exhibited a uniform applegreen fluorescence. In a reacted acrosome, only the equatorial segment of the acrosome was stained (Figure2) (23).
Reproducibility of host and acrosomal evaluations To evaluate the betweenobserver reproducibility of HOST, one slide from each donor was evaluated blindly by two observers. To determine the withinobserver reproducibility of HOST, the same slides were reevaluated blindly by one observer. The inter and intraobserver reproducibility of the acrosome scores in fresh and cryopreserved specimen were previously published (24). The average coefficient of variation between observers for acrosomal results was 6.5%. The intraclass correlation coefficient (ICC) between the observers was 0.81 [95% confidence interval (CI), 0.620.91]. The intraobserver coefficient of variation and the ICC for acrosomal evaluations were 1.6% and 0.98 (95% CI, 0.950.99), respectively.
Data are expressed as median and interquartile range. The Pearson method with an alpha level of 0.05 was used to correlate the viability results between hypoosmotic swelling test and Hoechst33258 staining before freezing and after thawing. Differences in the frequency of the acrosome reaction in viable spermatozoa according to the tail swelling or Hoechst 33258 pattern were evaluated by applying the Wilcoxon signedrank test. P < 0.05 was accepted as statistically different. Statistical analyses were performed using the SAS statistical software package (Cary, NC).
RESULTS
Sperm survival The nuclear dye Hoechst 33258 was considered as the gold standard to determine viability. The percentage of live spermatozoa in fresh and frozen specimens was 72.0% (64.5%87.0% interquartile range) and 29.5% (26.0%36.8% interquartile range), respectively. The percentage of spermatozoa exhibiting tail swelling after exposure to the hypoosmotic solution was 73.5% (66.0%85.5% interquartile range) in fresh and 50.0% (43.5%56.0% interquartile range) in frozen specimens.
In fresh specimens, the majority of viable spermatozoa, which fluoresced paleblue by Hoechst33258 staining, were also swollen by HOST (osmotically competent). The results of the HOST bly correlated with those obtained by Hoechst33258 staining (r = 0.95, p = 0.0001) (Figure4). After cryopreservation, we observed no correlation between the viability scores measured by HOST and Hoechst33258 staining (r = 0.11, p = 0.70) (Figure5). However, a small percentage of cryothawed spermatozoa were swollen before exposure to the hypoosmotic solution (median = 20.0% [18.0%23.0% interquartile range]). Even after correcting the HOST results for the swelling expected from cryopreservation, the viability scores measured by HOST and Hoechst 33258 stain showed poor correlation (r = 0.22; P = 0.43) (Figure6).
Acrosome reaction The evaluation of the acrosome reaction was performed by utilizing FITCPNA. Figure7 illustrates the importance of differentiating between normally reacted cells and post mortem degeneration of the acrosome. The percentage of cells exhibiting reacted acrosomes in fresh specimens was 28.0% (13.0%33.5% interquartile range). However, we observed a significant reduction in the frequency of reacted acrosomes when only viable spermatozoa, as assessed by Hoechst33258, were evaluated (median = 7.4% [2.0%10.9% interquartile range]; p < 0.001) (Figure7).
Utilizing both methods for assessing acrosome reaction in viable human spermatozoa, (1) FITCPNA and exposure to a hypoosmotic solution and (2) FITCPNA combined with Hoechst33258 stain, similar acrosome reaction rates could be detected in fresh specimens (median = 11.2% [5.9%15.2% interquartile range] versus 7.4% [2.0%10.9% interquartile range]; p = 0.07). In frozen specimens, the frequencies of acrosome reaction in viable spermatozoa assessed by FITCHoechst and FITCHOST were significantly different (median = 29.6% [23.1%33.3% interquartile range] versus 19.5% [16.0%24.5% interquartile range]; p = 0.01) (Figure8).
The average coefficient of variation between observers for HOST was 3.5%. The intraclass correlation coefficient (ICC) between the observers was 0.89 [95% confidence interval (CI), 0.760.99]. The coefficient of variation for duplicate evaluation of the same slides was 1.8%. The ICC between the two readings by the same observer was 0.93 (95% CI, 0.890.99).
COMMENTS
Standard semen analysis has limited predictive value for assessing the sperm fertilizing potential (25). Functional parameters of oocytes and spermatozoa are crucial for fertilization. Oocytes must be at the proper stage of maturity. Factors in spermatozoa include motility, membrane integrity, ability to bind to the zona pellucida, acrosin activity and membrane fusion ability, and also the acrosome reaction, which is of essential importance (12). Failed fertilization related to male factors, which occurs in 510% of invitro fertilization cycles and 23% of intracytoplasmic sperm injection cycles, may be observed in conjunction with apparent normal semen analysis (2,5). For these reasons, several functional tests have been proposed to explore sperm fertilization ability and to predict the success rate of IVF. Sperm morphology evaluated by strict criteria has been shown to be relevant (26). One of the most studied in the past was the zonafree hamster egg sperm penetration assay (SPA). Although good correlation with IVF have been reported, SPA does not represent a clinical suitable test because it cannot be performed routinely, it is expensive and timeconsuming, it gives some falsenegative responses, and it explores together several functions (capacitation, acrosome reaction and fusion to the oolema) (27). The ideal test system for sperm is IVF of human oocytes, which is properly governed by ethical constraints and cannot be used for a purely diagnostic purpose. Other tests such as hemizona assay, creatine kinase and the recent assays to examine sperm DNA fragmentation also seem to adequately assess the fertilizing potential of human sperm (7,28,29).
Overall, most sperm function tests are laborious and expensive, and they have yet to be proved clinically relevant for routine use in clinical andrology practice. Alternatively, the acrosome reaction (AR) test, which is a simple, inexpensive laboratory test that can be performed in any andrology laboratory with no restrictions associated with the availability of expertise or the testing material, has been shown to correlate well with fertilization (14,8,9). The AR test is based on sperm physiology. Mammalian spermatozoa must undergo a capacitation process before they are able to fertilize oocytes. Capacitation involves major biochemical and biophysical changes in the membrane complex and energy metabolism of the spermatozoa. Moreover, capacitation has been recognized as a timedependent phenomenon, with the absolute time course being speciesspecific. Capacitation prepares the sperm to undergo the acrosome reaction with the accompanying release of lytic enzymes and exposure of membrane receptors, which are required for sperm penetration through the zona pellucida and for fusion with the oolema (12). Integrity of acrosomal function seems to be of crucial importance to normal fertilization because acrosomeless roundheaded spermatozoa cannot fertilize oocytes, and increased percentages of morphologically abnormal acrosomes were related to IVF failure. Moreover, acrosome evaluation is also a valuable tool in modern andrology for both diagnosis of male infertility and research. Premature acrosome reaction and the inability of the spermatozoa to release the acrosomal contents in response to proper stimuli (acrosome reaction insufficiency) have been associated with idiopathic male infertility (30). Additionally, the development of contraceptive vaccines involving spermspecific antibodies that interfere in the acrosome reaction is one of the examples in the research field (10). Toxic potential of dietary substances and drugs can also be evaluated by AR assays. In a recent report, KumiDiaka & Townsend investigating the toxic potential of dietary isoflavones on sperm fertility have shown that despite of the fact that light microscopic could not identify detrimental effects of phytochemicals on sperm morphology, suppression of AR in higher doses and induction of AR at lower doses have been demonstrated with AR assays (11).
Therefore, many relevant aspects can be examined by studying the sperm acrosome and determination of the acrosome reaction, such as the true potential of spermatozoa for fertilization, the search for unexplained causes of male infertility and the possibility for male contraceptive development.
The human acrosome is a membranebound organelle, which appears during spermatogenesis as a product of the Golgi complex. It can be visualized by phase contrast light microscopy (18), and with greater accuracy by using electron microscopy, fluorescence (1,3,16,17,19), monoclonal antibodies (15), or simple dyes (13,14). However, electron microscopy and immunofluorescence do not differentiate between normally reacted cells and post mortem degeneration of the acrosome. Cross et al. (1986) employed supravital stain Hoechst 33258 (a fluorescent DNAbinding dye with limited membrane permeability) combined with immunofluorescence technique for evaluation of acrosome reaction in viable spermatozoa (17). They observed a discrepancy between viable spermatozoa (Hoechst 33258 negative), concerning the acrosome reaction, and the total number of acrosomereacted spermatozoa. Consequently, for exact evaluation of the acrosome reaction as a physiological process leading to fertilization, the determination of viable spermatozoa that have undergone acrosome reaction is important.
The determination of viability when studying the acrosome status in cryopreserved sperm is of fundamental importance. Cryopreservation directly damages sperm membrane, resulting in loss of membrane permeability and subsequent cell death (20). Cryopreservation can also cause permanent functional damage (sublethal damage), reducing the fertilizing ability of human sperm (19). This reduction in fertility can be explained partially by the reduction in the percentage of normal intact acrosomes and in total acrosin activity. Although damage to the acrosome after cryopreservation may also be secondary to cell death (20), an increase in the proportion of viable acrosomereacted spermatozoa after cryopreservation has been reported (19). These observations further stress the clinical importance of adequate assessment of the acrosomal status in cryopreserved sperm.
In the present study, we developed a protocol based on Aitken et al. previous work (16) that involved sperm incubation in a hypoosmotic solution, staining with Hoechst33258, and staining with FITCPNA. Hypoosmotic swelling test (HOST) was originally developed as a clinical test for human spermatozoa (21). The percentage of swollen sperm after incubation under hypoosmotic conditions reflect the percentage of spermatozoa with intact membranes, as it has been suggested that HOST can also assess sperm viability (31). In the present study, the viability results assessed by Hoescht33258 and HOST were highly correlated in fresh sperm. The hypoosmotic swelling test provided a simple, effective and convenient means of evaluating viability of spermatozoa that have been monitored for acrosome status. HOST has potential advantages over dye exclusion techniques (16). It is definitely a valuable alternative to more complex protocols involving the use of fluorochromes in fresh sperm.
On the other hand, our results fail to show correlation between viability by Hoescht33258 and HOST in freezethaw sperm, even after correcting the percentage of spermatozoa swelled due to the cryopreservation process. The poor specificity of HOST in detecting viable sperm in cryopreservedthawed sperm has been previously demonstrated (31). The reasons for that are unknown, but we speculate that sperm head and tail membranes have different liabilities to the freezethawing process. It may be possible that the determining factor for sperm survival after cryopreservation is the membrane integrity of sperm head, which is not assessed by HOST. FITCPNA labeling in conjunction with the HOST cannot accurately evaluate the acrosome reaction in viable cryopreserved human spermatozoa, and to date protocols involving the use of supravital stains have to be used in such cases.
CONCLUSIONS
Simultaneous assessment of acrosomal status using FITCPNA labeling in conjunction with HOST provides a simple but effective method for establishing the state of acrosomal membrane and to monitor viability in fresh human spermatozoa. However, FITCPNA labeling should not be used in conjunction with the HOST to accurately evaluate the acrosome reaction in viable cryopreserved human spermatozoa.
ACKNOWLEDGEMENT
Supported by The Cleveland Clinic Foundation Research Program Committee (grant no. 5490), Cleveland, Ohio, USA.
CONFLICT OF INTEREST
None declared.
Accepted after revision:
October 10, 2006
EDITORIAL COMMENT
The authors are to be commended for their efforts to simplify the technique of concurrently assessing acrosome status (reacted vs. nonreacted) and overall sperm viability. The combination of the two methods investigated, the Fluoresceinconjugated peanut agglutinin (FITCPNA) lectin labeling test and the Hypoosmotic swelling test (HOST), allows for the simultaneous assessment of acrosome status and overall sperm viability, thus averting the need for dualfilter microscopy. This approach proved to be accurate for fresh sperm, but not so for cryopreservedthawed sperm, where the HOST assay was found not to correlate with the gold standard test for sperm viability, Hoeschst 33258 staining. Interestingly, the authors found that even after correcting for sperm swelling expected from cryopreservation, the viability scores measured by HOST and Hoeschst 33258 staining still poorly correlated. As the authors state, this finding suggests that the determining factor for sperm survival after cryopreservation may be the integrity of the sperm head membrane, which is not assessed by HOST. These interesting observations by the authors' make their work exciting, possibly leading to new insights into the mechanisms of sperm viability after cryopreservation and thawing.
Dr. Robert Brannigan
Assistant Professor of Urology
Northwestern University Medical School
Chicago, Illinois, USA
Email: Rbrannigan@northwestern.edu
EDITORIAL COMMENT
This paper has investigated whether the hypoosmotic swelling test and FITCPNA allow simultaneous assessment of vitality of spermatozoa and their acrossomal status. This appears to be of particular interest since the simultaneous investigation provides evidence if acrossomal loss can be classified as physiological or degenerative. Fresh and cryopreserved samples have been used in this experimental investigation. The authors found that FITCPNA labeling in conjunction with morphological assessment of spermatozoa after simultaneous HOST facilitates effective evaluation of acrossomal status and viability of spermatozoa in fresh samples. However, this technique failed to prove reliable in cryopreserved samples.
This experimental study appears to be neat and well executed, methodological flaws cannot be detected. However, the number of investigated subjects and samples has been quite small.
It should be critically mentioned that sperm function tests do not always appear superior versus conventional semen analysis. In fact these tests are usually laborious and expensive in routine analysis and mostly do not result in therapeutic consequences for the clinical andrologist. Results from this and similar studies conclusively are of some theoretical nature.
Dr. Thorsten Diemer
Klinik und Poliklinik fur Urologie
Universitatsklinikum Giessen und Marburg
JustusLiebigUniversitat
Giessen, Germany
Email: Thorsten.Diemer@chiru.med.unigiessen.de
REPLY BY THE AUTHORS
We thank Professor Brannigan and Professor Diemer for their comments. We agree with Professor Diemer when he says that sperm function tests are usually laborious and expensive to be included in routine semen analysis. However, some of them are quite simple and inexpensive, and in general, they are better predictors of the male reproductive potential than conventional semen analysis. Additionally, sperm function tests certainly may be very helpful for the clinical andrologist. The assessment of sperm morphology by strict criteria, direct antisperm antibodies measurements and the tests to determine the occurrence of sperm DNA fragmentation, to cite a few, have been incorporated into the clinical practice in the recent years. These tests, which originated from the basic science, were validated as useful tools either to predict the male reproductive potential or to help the clinician define which therapeutic option is best for the infertile couple, i.e., assisted reproduction or conventional andrological treatments.
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Publication Dates
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Publication in this collection
29 Aug 2007 -
Date of issue
June 2007
History
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Accepted
10 Oct 2006 -
Received
10 Oct 2006