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IJRM 2019, 17(8): 557-566 |
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Heidari M M, Danafar A, Moezzi F, Khatami M, Talebi A R. The association between TNP2 gene polymorphisms and Iranian infertile men with varicocele: A case-control study. IJRM 2019; 17 (8) :557-566
URL: http://ijrm.ir/article-1-1622-en.html
URL: http://ijrm.ir/article-1-1622-en.html
Mohammad Mehdi Heidari * 
1, Amirhossein Danafar2 , Fahime Moezzi1 , Mehri Khatami1 , Ali Reza Talebi3
1, Amirhossein Danafar2 , Fahime Moezzi1 , Mehri Khatami1 , Ali Reza Talebi3
1- Department of Biology, Faculty of Science, Yazd University, Yazd, Iran.
2- Department of Biology, Ashkezar Islamic Azad University, Ashkezar, Yazd, Iran
3- Research and Clinical Center for Infertility and Department of Anatomy, Shahid Sadoughi University of Medical Sciences, Yazd, Iran.
2- Department of Biology, Ashkezar Islamic Azad University, Ashkezar, Yazd, Iran
3- Research and Clinical Center for Infertility and Department of Anatomy, Shahid Sadoughi University of Medical Sciences, Yazd, Iran.
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| Abstract (HTML) (2500 Views)
The prevalence of this disorder is about 15-20% among the general population (3). Despite all evidence, including alteration in testicular histology and normal function of Sertoli and Leydig cells and also changes in semen parameters that occur as a result of varicocele (4, 5), there is still a debate about the direct mechanism responsible for the impact of varicocele on spermatogenesis and male fertility potential (6-9).
One of the important factors in the process of fertilization and normal development of the embryo is sperm DNA integrity (10). Several studies have shown that infertile men compared with fertile men display higher levels of sperm DNA damages (11-15).
During spermiogenesis, the sperm nucleus will undergo a major rearrangement, in which the histones are replaced by positively charged protamines (PRMs). The replacement of histones by PRMs in sperm DNA is supported by other proteins such as transition nuclear proteins (TNPs) (16, 17). This event makes sperm DNA highly condensed and protects the sperm genome integrity that is important for normal sperm function and fertility (18, 19).
TNP2 gene is located on human chromosome 16p13.3 (20, 21). The pathogenic mutations in the PRM and TNP genes could be one of the reasons for these altered levels (19). Several studies have demonstrated that in men with varicocele, the sperm DNA integrity is significantly reduced and also the amount of DNA damage is increased compared with healthy controls (12, 13, 22).
Therefore, because of the critical role of TNPs and PRMs in sperm DNA integrity, these proteins could be one of the best goals for study in varicocele condition. So in this study, we decided to analyze the TNP2 gene mutations in Iranian infertile varicocele patients.
The varicocele diagnosis and blood sample collection were performed by the urologist from 2011 to 2015. Semen analysis was performed according to the WHO criteria (23). Sperm parameters are listed in Table I that include sperm count, rapid (grade a), slow (grade b), and non-progressive (grade c) motility, and sperm morphology. The mean age of infertile men with varicocele and normal controls was 28.3 ± 5.63 and 29.7 ± 6.14 (Mean ± SD), respectively, and were match to each other.
Peripheral Blood samples of patient and control groups were collected in EDTA-coated tubes in the Research and Clinical Center for Infertility, Shahid Sadoughi University of Medical Sciences, Yazd, Iran and were stored at -20ºC until analysis.
The rate of sperm nuclear chromatin condensation was measured via toluidine blue (TB) staining (1). In this procedure, air-dried sperm smears were fixed in fresh ethanol-acetone and then hydrolyzed in HCl. Then the samples were rinsed in distilled H2O and finally stained with TB. The scores of chromatin quality of spermatozoa according to this procedure, included 0, good chromatin; 1, mild abnormal chromatin; 2, severe chromatin abnormality (1) .So, spermatozoa with scores 1 and 2 were considered as TB+ or abnormal chromatin, score 0 as a TB- or spermatozoa with normal chromatin.
In situ acid-induced denaturation of sperm nuclear DNA were measured by Acridine Orange (AO) staining. In this staining, air-dried sperm smears were fixed in Carnoy’s solution and then each sample was stained in AO. Samples were evaluated on the fluorescent microscope. The green (normal double-stranded DNA) and orange/red (abnormally denatured DNA) fluorescence spermatozoa percentage were calculated according to the recommended method provided by Talebi et al (15).
Single strand conformation polymorphism (SSCP) technique was used to analyse the unknown mutations because it's a simple and sensitive procedure (26). All PCR products from cases and controls were analyzed by SSCP. For the SSCP analysis, 5 μl of the PCR products were mixed with 10 μl of SSCP loading buffer. The samples were denatured at 95ºC for 5 min and then rapidly cooled on ice to prevent renaturation; 10 μl of this mixture was loaded onto the polyacrylamide gels. The PCR products of exon 1 with a size of 440 bp was loaded onto 8% (w/v) polyacrylamide gel for 22 hours at 100V and 14mA, and the PCR products relating to exon 2 with a size of 127 bp were loaded onto 10% (w/v) polyacrylamide gel for 15 hours at 110V and 16mA. The gels were stained using the standard silver staining procedure to reveal the bands of single-strand DNA, and then the gels were wrapped in cellophane for preservation. Direct sequencing of DNA from samples with altered band pattern in the SSCP was done by a commercial agency (Macrogene Seoul, South Korea) to identify mutations.
Table I. Mean and standard deviation of sperm parameters of patients and participants
97-173/Table_1.jpg)
Table II. Primers used for amplification with PCR
97-173/Table_2.jpg)
In order to clarify the relationship between the two study groups, we used the Chi-square goodness-of-fit test, and the values of p < 0.05 were regarded as statistically significant. Also, a Chi-square test was performed for determining if the case and control groups demonstrate Hardy-Weinberg equilibrium. Odds ratio (OR) was calculated to measure the strength of the association observed. Multiple logistic regression analysis models were used to evaluate the haplotypes as possible risk factors. This statistical analysis was performed by SPSS (Statistical Package for the Social Sciences, version 20, SPSS Inc., Chicago, IL, USA).
3. Results
The results of aniline blue staining show that AB-reacted spermatozoa (AB+) rates in varicocele and control groups were significant (p ≤ 0.001). With regard to the AO test, DNA damage in sperm nuclei from infertile men with varicocele was a significant difference control group (p = 0.001). Also, the results of TB staining showed a significant difference between control and varicocele groups (p ≤ 0.001).
After the amplification of DNA fragments that isolated from blood samples of 156 patients and 150 controls using PCR and then SSCP procedures, some altered conformation patterns were detected by the SSCP analysis for the fragments of exons 1 & 2 of the TNP2 gene. Finally, the samples of these altered conformation patterns were sequenced (Figure 1). The results of sequencing showed three variants at positions g.IVS1-26 G>C (rs8043625), c.301C>T (rs34904070), and c.391C>T (rs11640138) of this gene. c.301C>T mutation changes the Arginine to Cysteine at position 101 (p.R101C) and c.391C>T changes the Arginine to Tryptophan at position 131 (p.R131W) of TP2 protein.
Genotype distribution in the control group for the all polymorphisms was in Hardy-Weinberg equilibrium. No significant differences were observed in genotype and allele frequencies of c.301C>T and c.391C>T variants. The distribution of genotype frequencies between Varicocele patients and controls wasn’t statistically significant, differences neither in the co-dominant nor in the dominant and recessive models (Tables III and IV). But for g.IVS1-26G>C SNP, the genotype frequencies of the G/G, G/C, and C/C were as 25.6%, 44.9%, and 29.5%, respectively, in cases and 50.7%, 37.3%, and 12%, respectively, in controls. The logistic regression analysis showed a significant association of the g.IVS1-26G>C SNP and Varicocele according to the dominant, recessive, and over-dominant models (dominant model OR: 2.98, 95% CI: 1.84-4.82; p = 0.000, recessive model OR: 3.07, 95%CI: 1.68-5.59); p = 0.000, and over-dominant model OR: 1.37, 95% CI: 0.86-2.16; p ≤ 0.001) (Table V).
Table VI shows the haplotype frequencies of three SNPs in two groups. The results of multiple logistic regression analyses revealed that the haplotypes (C/C/T) and (C/T/T) were a risk factor in patients with varicocele compared to controls (OR = 3.278, p ≤ 0.001, and OR = 9.304, p = 0.038, respectively).
Table III. Genotype distribution and relative allele frequencies of rs34904070 (c.301C>T) polymorphism in the TNP2 gene among Varicocele and control group
97-173/Table_3.jpg)
Table IV. Genotype distribution and relative allele frequencies of rs11640138 (c.391T>C) polymorphism in the TNP2 gene among Varicocele and control group
97-173/Table_4.jpg)
Table V. Genotype distribution and relative allele frequencies of rs8043625 (g.IVS1-26G>C) polymorphism in the TNP2 gene among Varicocele and control group
97-173/Table_5.jpg)
Table VI. Haplotype analysis of TNP2 polymorphisms with Varicocele patients and in controls
97-173/Table_6.jpg)
97-173/Figure_1.jpg)
Figure 1. (A) The SSCP patterns of exon 2 of TNP2 gene. (B) The results of direct sequencing of exon 2 of TNP2 gene revealed g.IVS1-26G>C (rs8043625). Lanes 3, 4, and 6 show G/G, C/C, and C/G genotypes, respectively. Also, lanes 1, 2, and 5 have G/G genotype and lane 7 similar to lane 6 has C/G.
Also, we identified the g.IVS1-26G>C (rs8043625) in the intronic region of this gene in both cases and controls that showed a significant difference in incidences between the patient and the control group. Siasi et al studied the relationship between polymorphisms of TNP2 gene with male infertility in 96 idiopathic infertile men with azoospermia or oligospermia and 100 normal control men in Iranian population. Their results show that the g.IVS1-26G>C was not associated with male infertility (34). Miyagawa et al evaluated the mutations of TNP1 and TNP2 genes in male infertility in the Japanese population. In this study, more than 10 SNPs were found in these genes in which the prevalence g.IVS1-26G>C in infertile males was not significantly different from that in fertile controls (35). However, biochemical analyses have proven that TNP2 increases the melting temperature of DNA and leads to DNA compacts to nucleosomal cores, which shows that it is a DNA-condensing protein (36). These analyses represent that this protein plays an important role in chromatin remodeling during spermiogenesis and for this reason, a few amino acid changes are tolerated in TNP2. However, the importance of TNP2 in human sperm formation is not fully understood. In our study, a three-dimensional structure model prediction of TP2 protein using the Protein Model Portal server has been made. The prediction of the tertiary structure of TP2 protein through in-silico analysis indicated that p.R101 and p.R131 are parts of a β strand located in a conserved region among several mammalian species (Figure 2). Predicted results of the pathogenicity of these variants with SIFT and PolyPhen tools are also summarized in Table VII. IVS1-26G>C is a known single nucleotide polymorphism that was identified in the intronic region of this gene (35). TNP2 sequence is poorly conserved during the evolution, and the levels of TNP2 expression and its protein vary among species (35). But the g.IVS1-26G>C polymorphism shows that they are conserved among other species and we also found a significant difference in the genotype and allele frequencies in patients with varicocele compared to controls. In addition, the haplotype analysis suggests combining genetic variations are associated with increased risk in patients with varicocele compared to controls (Table VI).
Table VII. Predicted results of the pathogenicity of rs34904070 (P.101 R>C) and rs11640138 (P.131 R>W) variants with SIFT and PolyPhen tools
97-173/Table_7.jpg)
97-173/Figure_2.jpg)
Figure 2. A three-dimensional structure model prediction of TP2 protein using the Protein Model Portal server and showing a close-up of the R101 (A) and C101 residues (B), R131 (C) and W131 (D) using PyMol.
Acknowledgments
This work was supported by the Yazd University. The authors would like to thank all the patients for providing blood samples for the scientific research and the Research and Clinical Center for Infertility (Yazd, Iran), whose cooperation was essential for this work.
Conflict of Interest
The authors declare that they have no conflict of interests.
Full-Text: (488 Views)
- Introduction
The prevalence of this disorder is about 15-20% among the general population (3). Despite all evidence, including alteration in testicular histology and normal function of Sertoli and Leydig cells and also changes in semen parameters that occur as a result of varicocele (4, 5), there is still a debate about the direct mechanism responsible for the impact of varicocele on spermatogenesis and male fertility potential (6-9).
One of the important factors in the process of fertilization and normal development of the embryo is sperm DNA integrity (10). Several studies have shown that infertile men compared with fertile men display higher levels of sperm DNA damages (11-15).
During spermiogenesis, the sperm nucleus will undergo a major rearrangement, in which the histones are replaced by positively charged protamines (PRMs). The replacement of histones by PRMs in sperm DNA is supported by other proteins such as transition nuclear proteins (TNPs) (16, 17). This event makes sperm DNA highly condensed and protects the sperm genome integrity that is important for normal sperm function and fertility (18, 19).
TNP2 gene is located on human chromosome 16p13.3 (20, 21). The pathogenic mutations in the PRM and TNP genes could be one of the reasons for these altered levels (19). Several studies have demonstrated that in men with varicocele, the sperm DNA integrity is significantly reduced and also the amount of DNA damage is increased compared with healthy controls (12, 13, 22).
Therefore, because of the critical role of TNPs and PRMs in sperm DNA integrity, these proteins could be one of the best goals for study in varicocele condition. So in this study, we decided to analyze the TNP2 gene mutations in Iranian infertile varicocele patients.
- Material & Methods
- Participants
The varicocele diagnosis and blood sample collection were performed by the urologist from 2011 to 2015. Semen analysis was performed according to the WHO criteria (23). Sperm parameters are listed in Table I that include sperm count, rapid (grade a), slow (grade b), and non-progressive (grade c) motility, and sperm morphology. The mean age of infertile men with varicocele and normal controls was 28.3 ± 5.63 and 29.7 ± 6.14 (Mean ± SD), respectively, and were match to each other.
Peripheral Blood samples of patient and control groups were collected in EDTA-coated tubes in the Research and Clinical Center for Infertility, Shahid Sadoughi University of Medical Sciences, Yazd, Iran and were stored at -20ºC until analysis.
- Semen analysis
- The assessment of sperm nuclear chromatin
The rate of sperm nuclear chromatin condensation was measured via toluidine blue (TB) staining (1). In this procedure, air-dried sperm smears were fixed in fresh ethanol-acetone and then hydrolyzed in HCl. Then the samples were rinsed in distilled H2O and finally stained with TB. The scores of chromatin quality of spermatozoa according to this procedure, included 0, good chromatin; 1, mild abnormal chromatin; 2, severe chromatin abnormality (1) .So, spermatozoa with scores 1 and 2 were considered as TB+ or abnormal chromatin, score 0 as a TB- or spermatozoa with normal chromatin.
In situ acid-induced denaturation of sperm nuclear DNA were measured by Acridine Orange (AO) staining. In this staining, air-dried sperm smears were fixed in Carnoy’s solution and then each sample was stained in AO. Samples were evaluated on the fluorescent microscope. The green (normal double-stranded DNA) and orange/red (abnormally denatured DNA) fluorescence spermatozoa percentage were calculated according to the recommended method provided by Talebi et al (15).
- Mutation screening of TNP2 gene
Single strand conformation polymorphism (SSCP) technique was used to analyse the unknown mutations because it's a simple and sensitive procedure (26). All PCR products from cases and controls were analyzed by SSCP. For the SSCP analysis, 5 μl of the PCR products were mixed with 10 μl of SSCP loading buffer. The samples were denatured at 95ºC for 5 min and then rapidly cooled on ice to prevent renaturation; 10 μl of this mixture was loaded onto the polyacrylamide gels. The PCR products of exon 1 with a size of 440 bp was loaded onto 8% (w/v) polyacrylamide gel for 22 hours at 100V and 14mA, and the PCR products relating to exon 2 with a size of 127 bp were loaded onto 10% (w/v) polyacrylamide gel for 15 hours at 110V and 16mA. The gels were stained using the standard silver staining procedure to reveal the bands of single-strand DNA, and then the gels were wrapped in cellophane for preservation. Direct sequencing of DNA from samples with altered band pattern in the SSCP was done by a commercial agency (Macrogene Seoul, South Korea) to identify mutations.
- Bioinformatics analysis
Table I. Mean and standard deviation of sperm parameters of patients and participants
Table II. Primers used for amplification with PCR
- Ethical consideration
- Statistical analysis
In order to clarify the relationship between the two study groups, we used the Chi-square goodness-of-fit test, and the values of p < 0.05 were regarded as statistically significant. Also, a Chi-square test was performed for determining if the case and control groups demonstrate Hardy-Weinberg equilibrium. Odds ratio (OR) was calculated to measure the strength of the association observed. Multiple logistic regression analysis models were used to evaluate the haplotypes as possible risk factors. This statistical analysis was performed by SPSS (Statistical Package for the Social Sciences, version 20, SPSS Inc., Chicago, IL, USA).
3. Results
The results of aniline blue staining show that AB-reacted spermatozoa (AB+) rates in varicocele and control groups were significant (p ≤ 0.001). With regard to the AO test, DNA damage in sperm nuclei from infertile men with varicocele was a significant difference control group (p = 0.001). Also, the results of TB staining showed a significant difference between control and varicocele groups (p ≤ 0.001).
After the amplification of DNA fragments that isolated from blood samples of 156 patients and 150 controls using PCR and then SSCP procedures, some altered conformation patterns were detected by the SSCP analysis for the fragments of exons 1 & 2 of the TNP2 gene. Finally, the samples of these altered conformation patterns were sequenced (Figure 1). The results of sequencing showed three variants at positions g.IVS1-26 G>C (rs8043625), c.301C>T (rs34904070), and c.391C>T (rs11640138) of this gene. c.301C>T mutation changes the Arginine to Cysteine at position 101 (p.R101C) and c.391C>T changes the Arginine to Tryptophan at position 131 (p.R131W) of TP2 protein.
Genotype distribution in the control group for the all polymorphisms was in Hardy-Weinberg equilibrium. No significant differences were observed in genotype and allele frequencies of c.301C>T and c.391C>T variants. The distribution of genotype frequencies between Varicocele patients and controls wasn’t statistically significant, differences neither in the co-dominant nor in the dominant and recessive models (Tables III and IV). But for g.IVS1-26G>C SNP, the genotype frequencies of the G/G, G/C, and C/C were as 25.6%, 44.9%, and 29.5%, respectively, in cases and 50.7%, 37.3%, and 12%, respectively, in controls. The logistic regression analysis showed a significant association of the g.IVS1-26G>C SNP and Varicocele according to the dominant, recessive, and over-dominant models (dominant model OR: 2.98, 95% CI: 1.84-4.82; p = 0.000, recessive model OR: 3.07, 95%CI: 1.68-5.59); p = 0.000, and over-dominant model OR: 1.37, 95% CI: 0.86-2.16; p ≤ 0.001) (Table V).
Table VI shows the haplotype frequencies of three SNPs in two groups. The results of multiple logistic regression analyses revealed that the haplotypes (C/C/T) and (C/T/T) were a risk factor in patients with varicocele compared to controls (OR = 3.278, p ≤ 0.001, and OR = 9.304, p = 0.038, respectively).
Table III. Genotype distribution and relative allele frequencies of rs34904070 (c.301C>T) polymorphism in the TNP2 gene among Varicocele and control group
Table IV. Genotype distribution and relative allele frequencies of rs11640138 (c.391T>C) polymorphism in the TNP2 gene among Varicocele and control group
Table V. Genotype distribution and relative allele frequencies of rs8043625 (g.IVS1-26G>C) polymorphism in the TNP2 gene among Varicocele and control group
Table VI. Haplotype analysis of TNP2 polymorphisms with Varicocele patients and in controls
Figure 1. (A) The SSCP patterns of exon 2 of TNP2 gene. (B) The results of direct sequencing of exon 2 of TNP2 gene revealed g.IVS1-26G>C (rs8043625). Lanes 3, 4, and 6 show G/G, C/C, and C/G genotypes, respectively. Also, lanes 1, 2, and 5 have G/G genotype and lane 7 similar to lane 6 has C/G.
- Discussion
Also, we identified the g.IVS1-26G>C (rs8043625) in the intronic region of this gene in both cases and controls that showed a significant difference in incidences between the patient and the control group. Siasi et al studied the relationship between polymorphisms of TNP2 gene with male infertility in 96 idiopathic infertile men with azoospermia or oligospermia and 100 normal control men in Iranian population. Their results show that the g.IVS1-26G>C was not associated with male infertility (34). Miyagawa et al evaluated the mutations of TNP1 and TNP2 genes in male infertility in the Japanese population. In this study, more than 10 SNPs were found in these genes in which the prevalence g.IVS1-26G>C in infertile males was not significantly different from that in fertile controls (35). However, biochemical analyses have proven that TNP2 increases the melting temperature of DNA and leads to DNA compacts to nucleosomal cores, which shows that it is a DNA-condensing protein (36). These analyses represent that this protein plays an important role in chromatin remodeling during spermiogenesis and for this reason, a few amino acid changes are tolerated in TNP2. However, the importance of TNP2 in human sperm formation is not fully understood. In our study, a three-dimensional structure model prediction of TP2 protein using the Protein Model Portal server has been made. The prediction of the tertiary structure of TP2 protein through in-silico analysis indicated that p.R101 and p.R131 are parts of a β strand located in a conserved region among several mammalian species (Figure 2). Predicted results of the pathogenicity of these variants with SIFT and PolyPhen tools are also summarized in Table VII. IVS1-26G>C is a known single nucleotide polymorphism that was identified in the intronic region of this gene (35). TNP2 sequence is poorly conserved during the evolution, and the levels of TNP2 expression and its protein vary among species (35). But the g.IVS1-26G>C polymorphism shows that they are conserved among other species and we also found a significant difference in the genotype and allele frequencies in patients with varicocele compared to controls. In addition, the haplotype analysis suggests combining genetic variations are associated with increased risk in patients with varicocele compared to controls (Table VI).
Table VII. Predicted results of the pathogenicity of rs34904070 (P.101 R>C) and rs11640138 (P.131 R>W) variants with SIFT and PolyPhen tools
Figure 2. A three-dimensional structure model prediction of TP2 protein using the Protein Model Portal server and showing a close-up of the R101 (A) and C101 residues (B), R131 (C) and W131 (D) using PyMol.
- Conclusion
Acknowledgments
This work was supported by the Yazd University. The authors would like to thank all the patients for providing blood samples for the scientific research and the Research and Clinical Center for Infertility (Yazd, Iran), whose cooperation was essential for this work.
Conflict of Interest
The authors declare that they have no conflict of interests.
Type of Study: Original Article |
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