| HOME | HELP | FEEDBACK | SUBSCRIPTIONS | ARCHIVE | SEARCH | TABLE OF CONTENTS |
,
,
From the * Unidad de Genética, Facultad de
Biología, Universidad Autónoma de Madrid, Spain;
Sección de Genética y Unidad de
Investigación, Complejo Hospitalario Universitario Juan Canalejo, As
Xubias, Coruña, Spain; ARGGORA Unidad
de la Mujer, A Coruña, Spain; Unidad de
Andrología, Servicio de Bioquímica, Hospital La Paz, Madrid,
Spain; and || Servicio de Andrología,
IVI-Madrid, Madrid, Spain.
| Correspondence to: Dr José Luis Fernández, Sección de Genética y Unidad de Investigación, Complejo Hospitalario Universitario Juan Canalejo, As Xubias, 84, 15006-A Coruña, Spain (e-mail: JLFernandez{at}canalejo.org or genetica{at}cog.es). |
| Received for publication June 27, 2005; accepted for publication September 6, 2005. |
 |
Abstract |
|---|
 Top Abstract Materials and MethodsResultsDiscussionReferences |
|---|
Key words: Human sperm, DNA fragmentation
Recently, a higher frequency of sperm cells with fragmented DNA has been reported in the ejaculate of subjects with varicocele, in comparison with fertile donors (Saleh et al, 2003; Chen et al, 2004). This phenomenon may be correlated with an increase of reactive oxygen species (ROS), resulting in oxidative stress (OS), which causes lipid peroxidation of sperm plasma membrane and nuclear DNA damage. Nitric oxide (NO) released by the endothelial cells from the dilated spermatic veins and the peroxynitrite generated by its reaction with the superoxide radical is probably an important source of such oxidative damage (Mitropoulos et al, 1996). DNA fragmentation may be a direct expression of this damage or a consequence of triggering of an apoptotic-like process by the ROS overproduction. These seminal abnormalities were also evidenced in experimental varicocele in rats, where enhanced ROS production and an increase in the sperm cells with fragmented DNA was demonstrated.
Enzymatic end-labeling with terminal nucleotidil transferase (TUNEL) or the sperm chromatin structure assay (SCSA) have been used to determine DNA fragmentation in sperm cells in subjects with varicocele. Recently, we developed a new technique, called sperm chromatin dispersion (SCD) test, as a simple procedure to analyze sperm DNA fragmentation (Fernández et al, 2003). The SCD has been improved and developed as the Halosperm® kit, to be used mainly with the conventional bright-field microscope (Fernández et al, 2005). Using this procedure, sperm cells, immersed on an agarose microgel on a slide, are incubated in an acid solution to transform DNA breaks into single-stranded DNA motifs, and then in a lysing solution to remove membranes and proteins. The resulting partially deproteinized nucleus, that is, the nucleoid, consists of a central core and a halo of dispersion of DNA loops. The sequential DNA breakage detection-fluorescence in situ hybridization (DBD-FISH) demonstrated that those sperm nuclei without fragmented DNA show big or medium-sized halos, whereas those containing DNA fragmentation appear with a small halo, without a halo and with a solid staining of the core, or without halo and irregular or faint staining of the core, that is, degraded. This consecutive pattern reflects a progressive higher yield of DNA-nuclear damage, as evidenced by the improved SCD test. Thus, the degraded-type corresponds to the strongest nuclear damage that also compromises the nuclear matrix, so possibly DNA and the residual proteins from the core result partially removed under the technical conditions.
We have determined the sperm DNA fragmentation, detailing the relative profile of different categories of DNA-nuclear damage resulting after the processing by the Halosperm® kit, in sperm cells from infertile patients with varicocele. The results have been compared with those from fertile men and those with idiopathic infertility, either from normozoospermic patients or from patients with abnormal standard semen parameters.
|
Materials and Methods |
|---|
|
TopAbstractMaterials and MethodsResultsDiscussionReferences |
|---|
SCD Test
The SCD test was developed as the Halosperm® kit (INDAS Laboratories,
Madrid, Spain). An aliquot of each sperm sample was diluted to 10 million/mL
in PBS. Gelled aliquots of low melting-point agarose in Eppendorf tubes are
provided in the kit, each 1 to process a semen sample. The Eppendorf tube was
placed in a water bath at 90°C to 100°C for 5 minutes to fuse the
agarose, and then in a water bath at 37°C. After 5 minutes incubation for
temperature equilibration at 37°C, 60 µL of the diluted semen sample
was added to the Eppendorf tube and mixed with the fused agarose. Twenty
microliters of the semen-agarose mix was pipetted onto an agarose precoated
slide, provided in the kit, and covered with a 22- x 22-mm coverslip.
The slide was placed on a cold plate in the refrigerator (4°C) for 5
minutes to allow the agarose to produce a microgel with the sperm cells
trapped. The coverslip was gently removed and the slide immediately immersed
horizontally in an acid solution, previously prepared by mixing 80 µL of
HCl from an Eppendorf tube in the kit, with 10 mL of distilled water, and
incubated for 7 minutes. The slides were horizontally immersed in 10 mL of the
lysing solution for 25 minutes. After washing 5 minutes in a tray with
abundant distilled water, the slides were dehydrated in increasing ethanol
baths (70%-90%-100%) for 2 minutes each and air dried. The slides may be
stored for several months in a tightly closed box in the dark, at room
temperature, or immediately stained for fluorescence or bright-field
microscopy. For the latter, the slide was horizontally covered with a mix of
Wright's solution (Merck, Darmstadt, Germany) and phosphate buffer solution
(Merck) (1:1) for 5 to 10 minutes, with continuous airflow. Then the slide was
briefly washed in tap water and allowed to dry. Strong staining is preferred
to easily visualize the periphery of the dispersed DNA loop halos. A minimum
of 500 spermatozoa per sample were scored under the 100x objective of
the microscope.
Scoring Criteria
The categorization of the different halo sizes is performed using the minor
diameter of the core from the own nucleoid as a reference to which the halo
width is compared. Five SCD patterns were established
(Fernández et al, 2005):
a) Sperm cells with large halos: those whose halo width is similar or higher
than the minor diameter of the core. b) Sperm cells with medium-size halos:
the halo size is between those with high and with very small halo. c) Sperm
cells with very small-size halo: the halo width is similar or smaller than one
third of the minor diameter of the core. d) Sperm cells without a halo. e)
Sperm cells without a halo-degraded: similar to d but weakly or irregularly
stained. Sperm cells with very small halos, without halos, and without
halo-degraded contain fragmented DNA. Nucleoids that do not correspond to
sperm cells were separately scored.
Statistical Analysis
All data were analyzed by using the SPSS package software. Statistical
analysis was carried out using nonparametric Mann-Whitney U test
(P < .01).
|
Results |
|---|
|
TopAbstractMaterials and MethodsResultsDiscussionReferences |
|---|
|
A different situation was revealed when the different patterns of sperm cells with fragmented DNA were evaluated. Specifically, the contribution of the sperm cells with the higher DNA-nuclear damage level, that is, the degraded type, to the whole population of sperm cells with fragmented DNA, was determined (the Table; the Figure). The proportion of the degraded cells in the total of sperm cells with fragmented DNA was 1 out of 4.2 (23.9 ± 12.9) in the case of varicocele patients, whereas it was 1 out of 8.2 to 9.7 in the normozoospermic patients (11.1 ± 9.9) (P < .0001), in the patients with abnormal sperm parameters (12.2 ± 8.3) (P < .0001), and in the fertile group (10.3 ± 7.2) (P = .001). Thus, this proportion was not statistically significant among the 3 later groups, but significantly higher in the group with varicocele.
|
|
Discussion |
|---|
|
TopAbstractMaterials and MethodsResultsDiscussionReferences |
|---|
Otherwise, the absence of significant differences in the frequency of sperm cells with fragmented DNA between the normozoospermic patients and the patients with abnormal semen parameters should be considered in relative terms. In a previous report, we found that a group of 23 oligoasthenoteratozoospermic patients showed a mean of 47.3% of DNA fragmentation level (Fernández et al, 2005), significantly higher than that from the normozoospermic patients. This suggests that the group with abnormal semen parameters is very heterogeneous, and probably those samples with more intense and combined abnormalities could have more frequency of sperm cells with fragmented DNA. Thus, differences in the DNA fragmentation level should be found depending on the relative contribution of certain subgroups to the whole group of patients with abnormal semen parameters.
The discrimination of different degrees of DNA fragmentation is a unique attribute of the SCD test. The sperm cells with fragmented DNA may show small halos of dispersion of DNA loops, exhibit no halo but a solid stained core, or no halo with a faint or irregularly stained core. This gradation pattern reflects a progressively stronger DNA-nuclear damage. The latter, that is, the degraded type, must also compromise the nuclear matrix because, under the initial SCD protocol, they appear pulverized in small fragments (Fernández et al, 2003). This fact, together with the lack of preservation of the tail, sometimes makes it difficult to accurately discriminate spermatozoa from other cell types. The new SCD protocol developed in the Halosperm® kit is much less aggressive than the previous one, with better chromatin preservation and retention of the sperm tail, for the accurate discrimination of this extreme type of nuclear damage. Within the population with fragmented DNA, the contribution of the sperm cells with small halo and those without halo but with solid staining of the core is similar between each of the 4 groups. Nevertheless, 1 out of 4.2 sperm cells with fragmented DNA belong to the degraded type, in the varicocele samples. This duplicates the proportion of that observed in the normozoospermic patients, the patients with abnormal semen parameters, and in the fertile men. In these groups, it was found that 1 out of 8.2 to 9.7 cells with fragmented DNA had an extreme level of nuclear damage. Overall, our study shows that the mean frequency of sperm cells with fragmented DNA is almost twofold higher in infertile than in fertile men. Nevertheless, the relative proportion of extremely damaged sperm cells in the whole population containing fragmented DNA seems low and independent of the fertility status, except in the varicocele group. Thus, the determination of the contribution of the degraded type to the population with fragmented DNA could perhaps orient to the presence of a varicocele, as a complementary adjunct test in the diagnostic study, as the proposed determination of ROS and total antioxidant activity in semen (Saleh et al, 2003; Allamaneni et al, 2004). Moreover, it could be of great interest to assess if varicocelectomy diminishes the frequency of sperm cells with fragmented DNA, as recently reported (Zini et al, 2005), as well as the relative contribution of those with extreme nuclear damage to this population.
The nature of the nuclear damage in the degraded type deserves further investigation in our laboratories. It could be related to a strong and prolonged exposure to DNA-nuclear-damaging factors. Not only the DNA, but the proteins, especially those from the nuclear matrix, would be affected, leading to an advanced lytic stage. An enhancement in OS, both due to an increase in ROS production and a decrease in the antioxidant capacity, has been reported in men with varicocele (Barbieri et al, 1999; Hendin et al, 1999). Moreover, the increase in seminal ROS levels seems correlated with varicocele grade (Allamaneni et al, 2004). This is a well-known factor that may induce DNA fragmentation either in vivo or in vitro (Agarwal et al, 2003). NO and peroxynitrite, a potent oxidant ROS, have been demonstrated to be produced in high concentrations in the dilated spermatic veins, so they could be main contributors to the high OS level in varicocele (Mitropoulos et al, 1996; Romeo et al, 2001; Turkyilmaz et al, 2004). Besides the dilated veins, ROS may be released in the seminiferous tubules by the cytoplasmic droplets retained in immature spermatozoa (Ollero et al, 2001), which seem to be frequent in the sperm samples from infertile men with varicocele (Zini et al, 2000). Immaturity is a consequence of defective spermiogenesis that could also lead to differences in disulfide crosslinking and in susceptibility toward DNA fragmentation.
Our results after incubating seminal samples with the NO donor sodium nitroprusside revealed a dose-response effect in the induction of DNA fragmentation, using the Halosperm® kit (Fernández et al, 2005). Nevertheless, this increase was due to those nucleoids with small halo and those without halo and solid staining of the core, those belonging to the degraded type remaining unchanged with respect to the untreated controls. This suggests that the ROS-induced DNA damage does not appreciably affect the architecture of the nuclear matrix. Nevertheless, this is an acute exposure, while the in vivo situation supposes a chronic OS, possibly mixed with cytokines and proteases, that may damage not only the DNA but also the nuclear proteins in a significant way. If this is the case, the relatively high frequency of sperm nuclei with the strongest nuclear damage level within the population of sperm cells with fragmented DNA may not only result from varicocele. Other pathologies, such as chronic infections or inflammatory processes, should be evaluated for this effect. Another possibility could be that this subgroup of spermatozoa is more susceptible to the ROS-induced nuclear damage, as previously cited. In fact, it has been reported that infertility due to male factor and those presenting varicocele may produce spermatozoa with less condensed chromatin (Molina et al, 2001), so ROS could have a better accessibility to the inside of these nuclei, producing a higher damage level. Independent of the mechanisms, our results indicate that the assessment of the relative profile of the different patterns of nuclear damage level, allowed by the SCD test, may be of great value in sperm analysis.
|
Acknowledgments |
|---|
|
Footnotes |
|---|
|
References |
|---|
|
TopAbstractMaterials and MethodsResultsDiscussionReferences |
|---|
Allamaneni SS, Naughton CK, Sharma RK, Thomas AJ Jr, Agarwal A. Increased seminal reactive oxygen species levels in patients with varicoceles correlate with varicocele grade but not with testis size. Fertil Steril. 2004;82: 1684 -1686.[CrossRef][Medline]
Barbieri ER, Hidalgo ME, Venegas A, Smith R, Lissi EA.
Varicocele-associated decrease in antioxidant defenses. J
Androl. 1999;20: 713
-717.
Chen C, Lee S, Chen D, Chien H, Chen I, Chu Y, Liu J, Chen W, Wu G.
Apoptosis and kinematics of ejaculated spermatozoa in patients with
varicocele. J Androl. 2004; 25: 348
-353.
Fernández JL, Lourdes M, Goyanes VJ, Segrelles E, Gosálvez J, Enciso M, Lafromboise M, De Jonge C. Simple determination of sperm DNA fragmentation with an improved sperm chromatin dispersion (SCD) test. Fertil Steril. 2005; 84: 833 -842.[CrossRef][Medline]
Fernández JL, Muriel L, Rivero MT, Goyanes V, Vázquez
R, Alvarez JG. The sperm chromatin dispersion test: a simple method for the
determination of sperm DNA fragmentation. J Androl. 2003; 24: 59
-66.
Hendin BN, Kolettis PN, Sharma RK, Thomas AJ Jr, Agarwal A. Varicocele is associated with elevated spermatozoal reactive oxygen species production and diminished seminal plasma antioxidant capacity. J Urol. 1999;161: 1831 -1834.[CrossRef][Medline]
Marmar JL. The pathophysiology of varicoceles in the light of
current molecular and genetic information. Hum Reprod
Update. 2001;7: 461
-472.
Mitropoulos D, Deliconstantinos G, Zervas A, Villiotou V, Dimopoulos C, Stavrides J. Nitric oxide synthase and xanthine oxidase activities in the spermatic vein of patients with varicocele: a potential role for nitric oxide and peroxynitrite in sperm dysfunction. J Urol. 1996;156: 1952 -1958.[CrossRef][Medline]
Molina J, Castilla JA, Castano JL, Fontes J, Mendoza N, Martinez L.
Chromatin status in human ejaculated spermatozoa from infertile patients and
relationship to seminal parameters. Hum Reprod. 2001; 16: 534
-539.
Ollero M, Gil-Guzmán E, Sharma RK, López MC, Larson
KL, Evenson DP, Agarwal A, Thomas AJ, Alvarez JG. Characterization of subsets
of human spermatozoa at different stages of maturation: implications in the
diagnosis and treatment of male infertility. Hum
Reprod. 2001;16: 1912
-1921.
Romeo C, Ientile R, Santoro G, Impellizzeri P, Turiaco N, Impala P, Cifala S, Cutroneo G, Trimarchi F, Gentile C. Nitric oxide production is increased in the spermatic veins of adolescents with left idiopathic varicocele. J Pediatr Surg. 2001; 36: 389 -393.[CrossRef][Medline]
Saleh RA, Agarwal A, Sharma RK, Said TM, Sikka SC, Thomas AJ Jr. Evaluation of nuclear DNA damage in spermatozoa from infertile men with varicocele. Fertil Steril. 2003; 80: 1431 -1436.[CrossRef][Medline]
Turkyilmaz Z, Gulen S, Sonmez K, Karabulut R, Dincer S, Can Basaklar A, Kale N. Increased nitric oxide is accompanied by lipid oxidation in adolescent varicocele. Int J Androl. 2004; 27: 183 -187.[Medline]
World Health Organization. WHO Laboratory Manual for the Examination of Human Semen and Semen-Cervical Mucus Interaction. Cambridge, United Kingdom: Cambridge University Press; 1999 .
Zini A, Blumenfeld A, Libman J, Willis J. Beneficial effect of
microsurgical varicocelectomy on human sperm DNA integrity. Hum
Reprod. 2005;20: 1018
-1021.
Zini A, Defreitas G, Freeman M, Hechter S, Jarvi K. Varicocele is associated with abnormal retention of cytoplasmic droplets by human spermatozoa. Fertil Steril. 2000; 74: 461 -464.[CrossRef][Medline]
| ||||||||||||||||||||||||||||||||||||||||||||||||||||||||||
| HOME | HELP | FEEDBACK | SUBSCRIPTIONS | ARCHIVE | SEARCH | TABLE OF CONTENTS |
