1 Reproductive Genetics Unit, Department of Obstetrics, Gynecology and Reproductive Sciences, Box 0720, University of California, San Francisco, CA 94143 and 2 Department of Anatomy and Reproductive Biology, University of Hawaii School of Medicine, Honolulu, Hawaii, 96822 USA
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Abstract |
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Key words: genomic imprinting/infertility/ROSI/spermatids
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Introduction |
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In mice, offspring have been reported following fertilization of oocytes with spermatids (Ogura et al., 1994; Kimura and Yanagimachi, 1995
). Initially the efficiency of producing liveborn offspring was low when the spermatids were fused to the oocytes, but this was dramatically increased when the spermatids were injected directly into the oocyte using a piezoelectric pipette-driving unit (Kimura and Yanagimachi, 1995
). Mice derived in this way develop normally and are fertile. Subsequent generations of mice originally derived from spermatids have been born and show no deleterious effects (Y.Kimura and R.Yangimachi, unpublished observations).
Given that the mice generated by spermatid injection appear normal, does it follow that imprinting in these mice is normal? Recent observations suggest that loss of genomic imprinting may be compatible at least with normal fetal and postnatal development. Chimeras created by the injection of Mus musculus/Mus spretus hybrid embryonic stem (ES) cells into Mus musculus blastocysts resulted in phenotypically normal chimeras that expressed imprinted genes bi-allelically in the hybrid cells (A.J.Villar, J.Gold, K.Mate, J.Meneses, J.McLaughlin, R.Pedersen, unpublished observations). Similarly, chimeras created with DNA methyltransferase / ES cells that had been rescued with a DNA methyltransferase transgene, resulted in healthy mice even though the contributing ES cells showed no imprinting (Tucker et al., 1996). In both of these cases, the ES cells constituted a high proportion of the chimeric tissues but no harmful effects from the presence of these abnormally imprinted ES cells were seen. Thus, absence of imprinting in the chimeric descendants of ES cells (which are known to contribute to fetal tissues but not to extra-embryonic endoderm and trophectoderm) appears to be compatible with normal development. By analogy, the apparently normal phenotype of spermatid-derived mice may not be informative about imprinting in the paternal gamete.
The injection of spermatids for the fertilization of human oocytes has recently been used as a treatment for severe male infertility, specifically in cases of incomplete maturational arrest of spermatogenesis leading to azoospermia (Tesarik and Mendoza, 1996; Tesarik et al., 1996
; Antinori et al., 1997
; Vanderzwalmen et al., 1997
). In order to evaluate the clinical relevance of spermatid injection it is important to address the imprinting status of spermatids in mammals. In addition to prenatal effects of any abnormalities in imprinting, there could be longer term effects. In humans some genetic diseases and tumour formation are associated with abnormal imprinting including SilverRussell, Albrights, PraderWilli and Angelmann's syndromes (Davies and Hughes, 1993
; Cassidy, 1995
; Williamson et al., 1996
; Eggermann et al., 1997
; Preece et al., 1997
). The overgrowth syndrome BeckwithWiedemann and Wilms' tumour are associated with improper imprinting of Igf-2 (Ogawa et al., 1993a
,b
; Rainier et al., 1993
; Weksberg et al., 1993
; Steenman et al., 1994
; Reik and Maher, 1997
). Moreover, relaxation of imprinting is found in some tumour cells (Brenton et al., 1995
).
Considering that the effects of abnormal imprinting might not be immediately apparent, it is important to establish the imprinting status of embryos created by round spermatid injection. The single nuceotide primer extension (SNuPE) assay is a polymerase chain reaction (PCR)-based assay which allows us to differentiate the levels of expression of two alleles of a gene with only a single base pair change. In order to use the SNuPE assay we needed to use strains of mice for our oocyte and round spermatid donors which had polymorphisms in imprinted genes. We have exploited interspecific polymorphisms between Mus castaneus and Mus musculus to assay quantitatively the expression of the paternally expressed genes Igf-2, Snrpn, and Peg1 (DeChiara et al., 1991; Leff et al., 1992
; Kaneko-Ishino et al., 1995) and the maternally expressed genes H19, Igf-2r and Mash2 (Barlow et al., 1991
; Bartolomei et al., 1991
; Guillemot et al., 1995
) from transcripts of embryos derived by spermatid injection.
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Materials and methods |
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Spermatid injections
Spermatid and sperm injections were carried out as described by Kimura and Yanagimachi (,Kimura and Yanagimachi, 1995b). Briefly, oocytes were isolated from the oviducts of superovulated B6D2F1 females 16 h post-human chorionic gonadotrophin (HCG) injection, cumulus cells removed with hyaluronidase treatment and kept in CZB medium (Chatot et al., 1989
, 1990
; Kimura and Yanagimachi, 1995
) at 37.5°C under 5% CO2 in air. Before spermatid injection, oocytes were activated with Ca2+-free CZB containing 5 mM SrCl2 for 30 min, then rinsed and cultured in CZB for 15 min. Round spermatids and epididymal spermatozoa were isolated from the seminiferous tubules of the testes and epididymis of Mus castaneus males (Jackson Laboratories) and suspended in HEPESCZB containing 8% polyvinylpyrrolidone (PVP) respectively. Injections were performed in HEPESCZB on a cooled (1718°C) stage using a piezoelectric pipette-driving unit (Model PMM-10, Prima Meat Packers, Tsuchiura Japan). A single spermatid nucleus was injected into an activated oocyte 15 to 45 min after SrCl2 treatment. As a control, an epididymal sperm head separated from the tail by application of a few piezo pulses was injected into an unactivated (metaphase II) oocyte. Injected oocytes were cultured in CZB. Oocytes containing two pronuclei were transferred to the oviducts of pseudopregnant recipients at the pronuclear or 2-cell stage and allowed to develop to mid-gestation stages or to term.
Isolation of RNA
Recipient females were killed and their embryos dissected at 10, 12 and 13 days of embryonic development. Embryos and extraembryonic tissue (including the amnion, yolk sac, allantois, and a portion of the chorion) were dissected in cold phosphate-buffered saline (PBS) and transferred to RNAzol B (Teltest Inc., Friendswood, TX, USA) on ice. Pools of four to 10 embryos or extraembryonic portions were frozen at 50°C in 3 ml RNAzolB. RNA was isolated following manufacturer's instructions and resuspended in diethyl pyrocarbonate (DEPC)-treated H2O.
SNuPE reaction
SNuPE reactions were carried out as described (Singer-Sam et al., 1992; Szabo and Mann, 1995
). To quantify allele-specific expression, reverse transcription of the embryonic and extraembryonic RNA samples was done as follows: reaction mix (1 µg RNA, 2.5 mM lower primer, 50 mM TrisHCl pH 8.3, 75 mM KCl, 3 mM MgCl2, 1 mM dNTP) was placed at 64°C for 10 min, 42°C for 15 min. 2.5 U/µl reverse transcriptase (RT; Superscript II, Gibco BRL) was added and the reaction continued at 42°C for 15 min. The reaction was stopped by heating to 99°C for 5 min, and finally held at 65°C. Controls without RT were done for each RNA sample to ensure that DNA was not amplified. Two microliters of cDNA were then added to a polymerase chain reaction (PCR) mix (20 mM TrisHCl pH 8.4, 50 mM KCl, 1.5 mM MgCl2, 200 mM dNTP, 0.5 mM lower and upper primers, 2.5 U/Rxn Taq DNA polymerase (Gibco, BRL). The reaction conditions were as follows: 94°C for 30 s, 42°C for 30 s, 72°C for 2 min (40 cycles), 72°C for 10 min followed by a 4°C soak for H19, Igf-2, Snrpn and Igf-2r, and 94°C for 45 s, 56°C for 45 s and 72°C for 1.5 min (40 cycles), 72 for 10 min followed by a 4°C soak for Peg1 and Mash2. PCR products were purified with Prep-A-Gene DNA purification Kit (BioRad). Approximately 10 ng of PCR product were added to the SNuPE reaction (20 mM TrisHCl pH 8.4, 50 mM KCl, 1.5 mM MgCl2, 2 µCi of the specific [32P]dNTP, 1 mM SNuPE primer, 0.75 U Taq DNA polymerase) and the reaction proceeded as follows: 4°C for 30 s, 42°C for 30 s, 72°C for 1 min. Electrophoresis through 12% polyacrylamide (BioRad) gels allowed SNuPE reaction visualization by autoradiography and quantification with a PhosphorImager. Specific [32P]dNTP added to each reaction were as follows: Peg-1 maternal (M)-dTTP, paternal (P)-dCTP; Snrpn M-dGTP, P-dATP; Igf-2 M-dCTP, P-dTTP; Igf-2r M-dATP, P-dGTP; H19 M-dATP, P-dCTP; Mash-2 M-dATP, P-dGTP.
RTPCR primers
The PCR primers used to produce a 197 bp fragment of Peg1 were as follows: upper primer (U), 5'-GCTGGGGAAGTAGCTCAGT-3'; lower primer (L), 5'-TTTCTTCTTAGCAAGGGCCA-3'; SNupePE primer (S), 5'-TTCAGTTCCAGCACTC-3'. Primers for H19, Igf-2, Igf-2r, and Snrpn were reported by Szabo and Mann (1995). For 474 bp H19 fragment: U, 5'-CCACTACACTACCTGCCTCAGAATCTGC-3'; L 5'-GGTGGGTACTGGGGCAGCATTG-3'; S 5'-ACATTCATACGGAGAGACTC-3'. For 235 bp Igf-2r fragment: U, 5'-CTGGAGGTGATGAGTGTAGCTCTGGC-3'; L 5'-GAGTGACGAGCCAACACAGACAGGTC-3'; S, 5'-TGCGGGGCCATC-3'. For 492 bp Igf-2 fragment: U, 5'-GACGTGTCTACCTCTCAGGCCGTACTT-3'; L, 5'-GGGTGTCAATTGGGTTGTTTAGAGCCA-3'; S, 5'-TCAAATTTGGTTTTTTAGAA-3'. For 356 bp Snrpn fragment: U, 5'-TGCTCGTGTTGCTGCTACTG-3'; L, 5'-GCAGTAAGAGGGGTCAAAAGC-3'; S, 5'-CAATTTCACAAGAAGCATT-3'. Sequences for PCR and SNuPE primers for Mash-2 PCR product were provided by Jeff Mann.
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Results |
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Spermatozoa injections
As a control for the injection procedure, oocytes in two replicates were injected with spermatozoa. Of the 113 oocytes injected, 17 oocytes lysed during the procedure. Of the 96 surviving oocytes, 89 (92.7%) were normally fertilized as indicated by two equally sized pronuclei. When these embryos were transferred at the pronuclear stage, 65 (73%) implanted and developed to at least day 10 at which time the pregnancies were terminated to collect fetal tissue (Table II).
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Analysis of paternally expressed genes
We investigated the allele-specific expression of the paternally expressed genes Snrpn, Igf-2 and Peg-1 in day 10, day 12 and day 13 spermatid-derived embryos and their extraembryonic tissues. As controls, we used C57BL/6J.CAST/Ei (N2) (F6) males which are homozygous for the Mus castaneus alleles at the distal 7 (Igf2 etc), proximal 7 (Snrpn etc), and proximal 17 (Igf2r) regions. Snrpn and Igf-2 are both located on mouse chromosome 7, but the Peg-1 gene is located on mouse chromosome 6. Since Mus castaneus chromosome 6 is not present in C57BL/6J.CAST/Ei (N2) (F6) males, we injected Mus castaneus spermatozoa into B6D2 F1 oocytes as an additional control. The sperm injection served as both a control for the injection procedure and gave us Mus castaneus/Mus musculus hybrid embryos at specific stages which are difficult to time with natural matings. Paternally expressed genes Snrpn, Igf-2 and Peg-1 were all found to be expressed exclusively from the paternal allele in embryos made by spermatid injection as well as control embryos from a normal mating, or in the case of Peg-1, from control embryos derived from sperm injection (Figure 1).
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The expression of Mash-2 in extraembryonic tissue was not exclusively maternal in our spermatid-derived embryos, as 1020% of the transcripts were from the Mus castaneus allele, which could only have come from spermatids. Expression of Mash-2 could not be detected in embryo RNA samples. However, the same quantitative pattern of expression characterized embryos derived from natural matings controls, indicating that this expression pattern was normal. We also detected 520% paternal expression of Igf-2r transcripts in all RNA samples both from experimental spermatid injection-derived embryos as well as natural mating controls (Figure 2).
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Discussion |
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By using the SNuPE assay to measure the expression of maternal and paternal alleles of imprinted genes, we have shown that imprinting appears normal for most imprinted genes tested in embryos derived from round spermatid injection. The three paternal genes, Igf-2, Snrpn and Peg-1, showed normal imprinting in the spermatid-injected embryos. This result was expected if the expression of the maternal copy of these genes had been repressed in the mature oocytes used. The maternal genes Igf-2r and Mash-2 both showed slightly leaky expression from the paternal alleles; however, this was also seen to the same extent in the controls. If the paternal genome had not been properly imprinted in spermatids we would have expected one of two results depending on whether the imprint was activating or repressing the genes being studied. In the case of repression, we would have expected completely bi-allelic expression (i.e. 50% of transcripts) of maternal genes in the absence of imprinting, but this was not observed. If the imprint resulted in activation of paternal genes, we would have expected to see an absence of paternal gene expression in the absence of imprinting. Again, this was not observed. Unlike the paternal expression of Igf-2r and Mash2, the leaky paternal expression of H19 seen with spermatozoa and round spermatid-injected embryos was not seen in embryos from normal matings. It has been shown in previous studies that H19 loses imprinting during in-vitro manipulations (Sasaki et al., 1995), which is consistent with our results. Only in one sample (day 12 extraembryonic tissue) did paternal H19 transcript levels even approach bi-allelic expression. In the remainder of samples, paternal H19 expression like that of Igf-2r and Mash2 was leaky rather than bi-allelic.
In principle, improperly imprinted genes in some of the embryos might have been masked by the pooling of the embryos. There was 1020% leakage seen in the maternal genes which could have been due to a single embryo with improper imprinting. However, this leaky paternal expression was also seen in the controls to a similar degree. In addition, our pools of embryos were small; pools of seven and 11 at day 10 and pools of five at day 12 and four at day 13. The sensitivity of the assay was such that even a single improperly imprinted embryo at day 12 and day 13 would have been detected, as well as detecting bi-allelic expression. Absence of expression of Igf-2 from improper imprinting would have resulted in abnormally small embryos (DeChiara et al., 1990, 1991
), and bi-allelic expression of Igf-2 results in larger embryos (Leighton et al., 1995
), neither of which was seen. However, overexpression of H19 and Snrpn has no phenotype (Pfeifer et al., 1996
). Mice with paternal disomy of the region of mouse chromosome 7 containing Snrpn appear normal (Cattanach et al., 1992
). All round spermatid-derived embryos at day 10, 12 and 13 appeared normal and of equal size.
Whereas expression of both maternal and paternal genes is seen in spermatids when assessed directly using the SNuPE method (Szabo and Mann, 1995), they are nevertheless properly imprinted as shown by correct parental-specific expression of the genes in the resulting embryos. Our results show that during normal gametogenesis, the correct paternal imprint is largely or entirely established by the spermatid stage, even though it may be labile in the case of H19. The ethical implications and possible consequences of the clinical use of ROSI to treat male infertility associated with severe testicular dysfunction continues to engender debate (reviewed by Aslam et al., 1998
; Sofikitis et al., 1998
). Potential clinical applications of spermatid injection in human oocytes will depend on whether imprinting will be normal in spermatids derived from males with abnormal spermatogenesis. Our results do not address the status of imprinting in the spermatids of the infertile male; this question therefore requires further study.
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Acknowledgments |
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Notes |
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References |
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Submitted on June 23, 1998; accepted on January 18, 1999.