1 Department of Urology, Universitätsklinikum Benjamin Franklin, Freie Universität Berlin, Hindenburgdamm 30, 12200 Berlin and 2 Department of Andrology, University of Hamburg, Hamburg, Germany
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Abstract |
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Key words: fertility/human telomerase reverse transcriptase/human telomerase RNA/spermatogenesis
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Introduction |
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Even the gold standard for assessing testicular tissue specimens, i.e. diagnostic testicular biopsy with histological work-up, is not a highly accurate parameter for detecting and classifying spermatogenesis (Silber et al., 1997). An approach for improving the diagnostic value of testicular biopsies is the molecularbiological detection of germ cell-specific gene expression.
A promising diagnostic parameter is the ribonucleoprotein telomerase, which functions as a cellular reverse transcriptase that catalyzes the synthesis and extension of telomeres (Greider and Blackburn, 1987). Most human somatic cells lose telomeric nucleotides with each cell division, which limits the number of cell divisions (Harley et al., 1990
). In contrast, germline, stem and more than 90% of tumour cells are believed to be immortal because telomere length is maintained by the action of telomerase (Kim et al., 1994
), which progressively adds hexamer TACGGGs repeats to the end of human chromosomes. Major components of the enzyme are the RNA template human telomerase RNA (hTR) (Feng et al., 1995
) and the catalytic subunit, human telomerase reverse transcriptase (hTERT) (Harrington et al., 1997
; Kilian et al., 1997
; Meyerson et al., 1997
; Nakamura et al., 1997
).
hTERT mRNA is expressed almost exclusively in germ cells, stem cells and malignant tumours and correlates closely with the detection of telomerase activity (Harrington et al., 1997; Kilian et al., 1997
; Meyerson et al., 1997
; Nakamura et al., 1997
). In contrast, hTR is expressed in benign and malignant tissue and correlates only loosely with the detection of telomerase expression (Feng et al., 1995
).
Several study groups have recently shown that the detection of telomerase activity in testicular biopsies is a helpful parameter for assessing disorders of spermatogenesis (Fujisawa et al., 1998; Yamamoto et al., 1999a
; Schrader et al., 2000a
).
We have also been able to show that the hTERT mRNA encoding for the catalytic subunit of telomerase in testicular tissue is a highly sensitive and specific marker for detecting germ cells in the testicles of men with non-obstructive azoospermia (Schrader et al., 2000a). The objective of the present study was to evaluate the quantitative detection of hTERT mRNA by real-time fluorescence RTPCR as a new molecular diagnostic parameter in the work-up of testicular tissue specimens from patients presenting with non-obstructive azoospermia.
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Materials and methods |
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Processing of testicular biopsy material
The tissue samples were subdivided into seven fractions, and the largest part (three fractions) was immediately placed in 1.0 ml of Sperm-Freeze® solution (Medicult, Hamburg, Germany) and transferred to liquid nitrogen by a computer-controlled system (Planer 10®; Messer-Griesheim, Griesheim, Germany).
One sample of testicular tissue from each patient was placed in a Petri dish containing Sperm-Prep® solution (Medicult) and examined within 10 min. Minced tissue was examined by phase-contrast microscopy at x400 magnification to detect cells of spermatogenesis, especially mature spermatids. In the case of negative findings, tissue was treated with collagenase type I (Sigma, Heidelberg, Germany) following a modified form of the protocol published by Schulze (Schulze and Knuth, 1998).
In one part of the sample, the expression of hTERT was quantitatively determined by fluorescence real-time RTPCR. The part intended for this was shock-frozen immediately after removal (35 min) and then stored in liquid nitrogen.
Another part of the sample was placed in Stieve's solution [formaldehyde DAB 10 20.0 g, acetic acid 100% DAB 10 4.0 g, aqueous saturated 7% mercuric (II) chloride solution 76.0 g per litre distilled H2O], paraffin-embedded and prepared in 5 µm slices. The slices were stained using haematoxylineosin (HE). The biopsy material was histologically evaluated according to the Johnsen score (JS) (Johnsen, 1970).
When assessment of the HE slices did not correspond to that of the wet preparation and/or the germ-cell-specific hTERT expression, tissue samples were also prepared using the semithin sectioning technique (Holstein, 1999). This procedure was also performed in all samples with spermatogenetic arrest and SCOS.
RNA extraction
Total RNA was extracted using the RNAzolB® extraction kit (WAK-Chemie Medical, Bad Homburg, Germany) according to the manufacturer's instructions, and its quality was assessed as previously described (Schrader et al., 2000a). RNA was treated with DNase (Amersham Pharmacia Biotec, Freiburg, Germany). The RNA yield was quantified by UV spectrophotometry. One microgram of total RNA was subjected to 1% agarose gel electrophoresis. Preservation of 28S and 18S rRNA species was used to assess RNA integrity. Samples without detection of 28S/18S RNA were excluded from further examination.
Quantitative detection of human telomerase catalytic subunit (hTERT) messenger RNA
Quantitative detection of hTERT mRNA was performed with the commercially available LightCycler® Telo TAGGG hTERT Quantification Kit® (Rouche Diagnostics GmbH, Mannheim, Germany) using the LightCycler® instrument (Roche Molecular Systems, Alameda, CA, USA) for on-line PCR and all subsequent quantification steps, according to the manufacturer's instructions.
The recently introduced LightCycler® (Wittwer et al., 1997a) is a thermocycler with on-line monitoring of PCR. The amplicon is detected by fluorescence using two short oligonucleotides that hybridize to an internal sequence of the amplified fragment during the annealing phase of the PCR cycles. One probe is labelled with a fluorescent dye at the 5' end, the other with fluorescein at the 3' end. The probes are designed to hybridize to the target strand so that the two dyes are in close proximity and fluorescence resonance energy transfer takes place between the two fluorophores. This leads to the emission of fluorescence, which is detected on-line during the PCR cycles.
The linear measuring range of the assay was set at 102106 copies by the manufacturer in an exemplary system using in-vitro transcribed hTERT mRNA. Our use of the provided in-vitro transcribed hTERT RNA as a reference showed the applied kit to have a sensitivity of approximately 100 hTERT mRNA copies. This high sensitivity of real-time fluorescence RTPCR with the LightCycler® has also been described by many other groups (Emig et al., 1999; Kreuzer et al., 1999
; Nakanishi et al., 1999
,2000
; Bolufer et al., 2000
; Simpson et al., 2000
) and is comparable to results obtained on other real time PCR equipment (Nitsche et al., 1999
).
hTERT- and the housekeeping gene porphobilinogen deaminase (PBGD)- mRNA specific primers span exonintron boundaries to prevent co-amplification of genomic DNA. Moreover, the primers have been selected so that one primer of both pairs is also used to prime reverse transcription (`gene-specific'). Thus only the specific targets are reverse-transcribed, which helps to increase the specificity of the assay.
Quantification of hTERT mRNA using the LightCycler® as a `one-step' closed tube system requires no post-amplification manipulation, resulting in short turnover times for data acquisition and analysis and minimizing hands-on time. A typical RTPCR to quantify hTERT gene expression in 12 patient samples took only 45 min on the LightCycler® instrument.
Briefly, hTERT encoding mRNA was reverse-transcribed (10 min at 60°C), followed by denaturation of the RNA/DNA complex (30 s at 95°C) and amplification of a 198 bp fragment of the generated cDNA in 40 PCR cycles (0.5 s at 95°C; 10 s at 60°C; 10 s at 72°C) with specific primers in a one-step RTPCR reaction. The following were prepared for each PCR assay: 2 µl of hTERT reaction mix, 0.1µl of reverse transcriptase, 2µl of hTERT or PBGD detection mix, 13.9 µl of H20 and 2 µl of standard RNA template (15)/100ng/1 µl of total RNA from an hTERT-positive cell line/H20 or sample RNA.
PTPCR for mRNA encoding the housekeeping gene for porphobilinogen deaminase (PBGD) was equally processed in separate tubes. The reaction product served as a control for RTPCR and as a reference for relative quantification of hTERT mRNA and hTR.
To carry out a positive control and establish an external standard curve, all measurements included the determination of five standards with in-vitro transcribed hTERT mRNA containing 1.3x106, 9.8x104, 8.0x103, 7.2x102 and 1.4x102 copies/2 µl as well as total RNA purified from an hTERT mRNA-expressing cell line provided by the detection kit. The graph of the linear regression and calculation of the regression coefficient r served to confirm the accuracy and reproducibility of this approach.
The total RNA served as a positive control for detection of PBGD mRNA. Probes without template that otherwise fulfilled the same requirements were examined as negative controls. Each sample was normalized on the basis of its PBGD content according to the formula NhTERT = hTERT mRNA copies sample/(PBGD mRNA copies sample /1000).
Probes were evaluated as hTERT mRNA-positive when the measurement of standard probes and controls yielded adequate results and >400 copies of PBGD mRNA were detected, suggesting an appropriate initial quantity and quality of total RNA. They were assessed as negative when no hTERT mRNA was detected in the presence of >400 copies of PBGD mRNA.
Statistical analysis
Statistical analysis was performed using the non-parametric KruskalWallis ANOVA on ranks test to compare the histological subgroups. A discriminant analysis of NhTERT was also performed for the different histological subgroups. Values were expressed as follows: mean, standard deviation, median, 25th percentile, 75th percentile and range. Statistical analysis was performed using SPSS software.
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Results |
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Testicular biopsies of patients with normal spermatogenesis
In 17 patients, testicular biopsy revealed histological evidence of full spermatogenesis. Tissue samples in all these cases were characterized by high hTERT mRNA expression with a mean NhTERT = 136.1 ± 41.7 copies (range 246.780.5). Fifteen of 17 tissue samples with evidence of full spermatogenesis had an hTERT mRNA expression of NhTERT >100 copies. Two tissue samples with only focally full spermatogenesis had an hTERT mRNA expression of NhTERT = 80.5 and 82.6 copies, which was in the range of tissue samples with maturation arrest.
Two specimens with an hTERT expression of NhTERT = 100.5 and 80.5 showed maturation arrest at the conventional histological work-up. Subsequent assessment by semithin sectioning disclosed focal islands with full spermatogenesis in both of these specimens.
Testicular biopsies of patients with maturation arrest
Twenty testicular biopsies revealed partial tubular atrophy with maturation arrest.
Among these were 16 tissue samples in which semithin sectioning provided histological evidence of spermatogenesis arrest at the primary and secondary spermatocyte level. In these cases, tissue samples showed a mean NhTERT expression of 53.8 ± 16.9 copies (range 83.927.1).
Four tissue samples evidenced spermatogenesis arrest at the level of the spermatogonia. These samples had a mean NhTERT expression of 16.4 ± 6.2 copies (range 25.011.2).
hTERT expression (NhTERT range 31.211.2 copies) was detected in four tissue specimens even though they evidenced SCOS at the histological work-up. The subsequent work-up by semithin sectioning revealed spermatocytes in two cases (NhTERT = 31.2 and 30.8 copies) and spermatogonia only in two others (NhTERT = 11.2 and 14.2 copies).
Testicular biopsies of patients with SCOS
In 12 patients, the histological work-up revealed germ cell aplasia.
Tissue samples with SCOS showed only minimal hTERT expression (NhTERT = 2.7 ± 2.8 copies; range 0.007.20). Figure 1 shows representative results of normalized hTERT expression in the different histological subgroups. Table II
gives a summary of histological findings and the expression of NhTERT in testicular biopsies.
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Discussion |
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Several study groups have recently shown that the detection of telomerase activity in testicular biopsies is helpful for detecting germ cells, particularly in patients with hypergonadotrophic hypogonadism with a predominant SCOS histology (Fujisawa et al., 1998; Yamamoto et al., 1999a
; Schrader et al., 2000b
).
The procedure applied by the above study groups was methodologically problematic inasmuch as the determination of telomerase activity by the telomeric repeat amplification protocol (TRAP) is influenced by numerous variables that impede an exact quantification. Although the TRAP assay has internal controls for PCR inhibition and telomerase activity, it does not check for variances in the telomerase yield due to cell lysis or instability of the enzyme activity during storage. Moreover, the TRAP assay only partially detects enzyme inhibition by tissue inhibitors and enzyme inactivation with heat or time.
Recently, we were able to demonstrate that the hTERT mRNA encoding for the catalytic enzyme component in testicular tissue is highly specific and highly sensitive for the presence of germ cells (Schrader et al., 2000a).
This study was the first to quantify hTERT mRNA by real-time fluorescence RTPCR in testicular tissue specimens from patients with various spermatogenesis disorders for which we intended to establish a molecular diagnostic subclassification. We chose this assay to avoid the above-mentioned problem in achieving an exact telomerase quantification by the TRAP assay. The advantage of this indirect detection procedure is that it accounts for varying tissue degradation with amplification of a housekeeping gene, and primary purification of RNA rules out tissue inhibitors of the PCR.
Moreover, it has repeatedly been shown that hTERT mRNA, in contrast to hTR, is rate-limiting for telomerase and that hTERT mRNA expression correlates well with telomerase activity (Harrington et al., 1997; Kilian et al., 1997
; Meyerson et al., 1997
; Nakamura et al., 1997
).
Quantification of hTERT mRNA with the LightCycler® shows numerous advantages in this connection.
For one thing, real-time online RTPCR has higher sensitivity compared to other quantification methods such as Northern blotting with in-situ hybridization (Parker and Barnes, 1999) or RNase protection assays (Hod, 1992
; Saccomanno et al., 1992
). Of practical importance is the fact that this non-radioactive method can start from less than 10 cells to obtain sufficient signals (Wittwer et al., 1997b
). A further advantage of the LightCycler® is the `real-time' technique. The fluorescence readings taken at every cycle of the PCR reaction are displayed immediately after each measurement, allowing amplification runs to be terminated or extended, as considered appropriate during individual runs. Real-time RTPCR also has the advantage of being significantly less variable than conventional RTPCR procedures (Bustin, 2000
). Zhang et al. showed that the coefficient of variation for Ct data is as low as 0.40.8% for the LightCycler®, which is significantly better than the 14% reported for conventional RTPCR (Wittwer et al., 1997b
; Zhang and Byrne, 1997
; Zhang et al., 1997
).
In 23 cases, the histological examination disclosed full spermatogenesis. All specimens showed high hTERT expression of NhTERT = 136.1 ± 41.7 copies. Two of the 17 specimens with reduced spermatogenesis and only focally full spermatogenesis had an hTERT expression of only NhTERT = 80.5 and 80.7 copies and were thus within the range of tissue samples with maturation arrest.
Maturation arrest was diagnosed in 20 specimens. Tissue samples with a JS of 35 had a mean hTERT expression of NhTERT = 48.2 ± 21.0 copies. Four tissue samples with maturation arrest at the level of spermatogonia (JS 3) had a markedly lower hTERT expression (NhTERT = 17.9 ± 5.3 copies) than those with a JS of 45 (NhTERT = 52.7 ± 10.2 copies).
Two tissue specimens with histologically diagnosed maturation arrest (JS 45) evidenced an hTERT expression of NhTERT = 80.5 and 105.0 copies, which was far above the mean value in the other specimens with MA. Other sections of the same tissue examined by the semithin sectioning technique showed focal islands of full spermatogenesis, which indicates that quantitative hTERT determination could contribute to a validation of histopathological findings.
Tissue specimens with SCOS showed only minimal hTERT expression with a mean of NhTERT = 2.7 ± 2.8 copies. In three tissue specimens that evidenced SCOS in the conventional histological work-up but had hTERT mRNA expression (NhTERT = 11.214.5 copies), spermatogonia were found in a renewed histological work-up by the semithin sectioning technique. This indicates that quantitative hTERT determination is highly sensitive and highly specific for detecting germ cells in testicular tissue specimens. Discriminant analysis showed that its determination in tissue samples had a high predictive value (89.0%) for correct classification in one of the three histological subgroups.
The markedly higher hTERT mRNA expression we detected in tissue specimens with full spermatogenesis may be due to the different expression level of hTERT mRNA in the telomerase-positive cells, i.e. spermatogonia, primary and secondary spermatocytes and round spermatids, depending on the spermatogenesis disorder.
The considerably higher hTERT gene expression in tissue specimens with full spermatogenesis would thus be partially attributable to the fact that comparable germ cells, e.g. spermatocytes, have markedly higher hTERT expression in specimens with full spermatogenesis than in those with spermatogenesis arrest at the level of primary or secondary spermatocytes. This is supported by studies of Yamamoto et al. (Yamamoto et al., 1999b) showing that telomerase profiles tend to be smaller in highly purified fractions of primary spermatocytes recovered from mice with primary testicular damage than in those recovered from healthy mice.
Moreover, a number of studies have demonstrated that hTERT mRNA expression shows marked variation in telomerase-positive cells, the different regulatory mechanisms including the cell cycle (Greenberg et al., 1998; Koyanagi et al., 2000
), hormones (Kyo et al., 1999
), cytokines (Uchida et al., 1999
; Xu et al., 2000
) and many other control mechanisms (Liu et al., 1999
; Nakamura et al., 1999
; Wick et al., 1999
; Harada et al., 2000
; Latil et al., 2000
). This suggests that similar regulatory mechanisms may be responsible for the different expression levels we observed in relation to the histological findings.
The increased hTERT expression in testicular tissue specimens may also be explained by the larger number of telomerase positive germ cells (e.g. spermatogonia, primary and secondary spermatocytes and round spermatids) per testis weight unit in patients with full spermatogenesis than in those with maturation. This hypothesis is supported by the study of Mio et al., which demonstrated a larger number of primary spermatocytes per testicular weight unit in Klinefelter men who are positive for haploid germ cells than in those who are positive for primary spermatocytes but negative for haploid germ cells (Mio et al., 1998).
The results of the present study show that hTERT mRNA expression in testicular tissue is highly sensitive and specific for germ cell activity and that its quantitative determination by real-time fluorescence RTPCR enables a molecular-diagnostic classification of spermatogenesis disorders. Thus quantitative determination of hTERT mRNA expression in testicular tissue appears to be well suited for predicting successful sperm recovery in patients with non-obstructive azoospermia and is a useful objective molecular diagnostic parameter for supplementing the histopathological evaluation. Our investigations show that an hTERT expression of NhTERT < 90 copies indicates full spermatogenesis, while maturation arrest without full spermatogenesis may be assumed at values of NhTERT < 70 copies. In the grey range of NhTERT = 70 < 90 copies, the diagnosis of maturation arrest should be checked by a further work-up of the specimens.
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Acknowledgements |
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Notes |
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References |
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Submitted on May 21, 2001; accepted on October 1, 2001.