Spatial Separation of Parental Genomes in Preimplantation Mouse Embryos

doi:10.1083/jcb.148.4.629

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© The Rockefeller University Press, 0021-9525/2000//629 $5.00
The Journal of Cell Biology, Volume 148, Number 4, , 2000 629-634

Brief Report

Spatial Separation of Parental Genomes in Preimplantation Mouse Embryos

Wolfgang Mayer^a, Avril Smith^a, Reinald Fundele^a, and Thomas Haaf^a

^a Max-Planck-Institut für Molekulare Genetik, 14195 Berlin, Germany
Max-Planck-Institute of Molecular Genetics, Ihnestrasse 73, 14195 Berlin, Germany.(49/0) 30 8413 1383(49/0) 30 8413 1251

haaf{at}molgen.mpg.de

We have used two different experimental approaches to demonstratetopological separation of parental genomes in preimplantationmouse embryos: mouse eggs fertilized with 5-bromodeoxyuridine(BrdU)-labeled sperm followed by detection of BrdU in earlydiploid embryos, and differential heterochromatin staining inmouse interspecific hybrid embryos. Separation of chromatinaccording to parental origin was preserved up to the four-cellembryo stage and then gradually disappeared. In F1 hybrid animals,genome separation was also observed in a proportion of somaticcells. Separate nuclear compartments during preimplantationdevelopment, when extreme chromatin remodelling occurs, andpossibly in some differentiated cell types, may be associatedwith epigenetic reprogramming.

Key Words: 5-bromodeoxyuridine • fluorescence in situ hybridization • mouse interspecific hybrids • nuclear architecture • preimplantation embryo

Introduction

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

An enormous body of data from classical genetics (Cattanach and Kirk 1985),nuclear transplantation experiments (McGrath and Solter 1984;Surani et al. 1986), and human imprinting disorders (Lalande 1996;Hall 1997) suggests that normal mammalian development requiresthe participation of both a maternal and a paternal genome.Opposing patterns of gene expression from maternally and paternallyderived alleles of imprinted genes explain the importance ofhaving both parental genomes for normal embryonic development(Fundele and Surani 1994; Tilghman 1999).

The one-cell embryo is formed from two very different sets ofchromatin: the highly compact, transcriptionally totally inertsperm DNA, and the maternal egg chromatin. Dramatic chromatinremodeling and reprogramming of developmental programs occurin the early mammalian embryo, resetting the differential gameticmarks into their functional forms. Ovulated oocytes appear tobe globally undermethylated, whereas the sperm genome is relativelymethylated. A genome-wide demethylation during preimplantationdevelopment leads to indistinguishable alleles at most geneloci, but not at those that are imprinted (Howlett and Reik 1991;Olek and Walter 1998). Although a net demethylation could becaused by a combination of undermethylated maternal and methylatedpaternal DNA (Monk et al. 1987; Sanford et al. 1987), accumulatingexperimental evidence suggests that overall changes in methylationlevels during early development may be the sum of highly dynamicand, maybe, differential processes in parental genomes (Yoder et al. 1997;Rougier et al. 1998; Mayer et al. 2000).

The oocyte is stocked with maternal mRNAs and proteins thatare required for the development of the one-cell embryo. Inthe mouse embryo, major activation of the zygotic genome beginsat the two-cell stage (Schultz 1986). However, minor gene transcriptionoccurs in the late one-cell embryo on already replicated DNA.Both replication and transcription are initiated earlier inthe male pronucleus, which is also less condensed than the femalepronucleus (Bouniol-Baly et al. 1997). Reporter gene transfectionexperiments (Wiekowski et al. 1993) and BrUTP incorporationassays (Aoki et al. 1997) showed a greater transcriptional activityin the male pronucleus. Activation of the male pronucleus maydepend on transient histone H4 hyperacetylation of paternalDNA (Adenot et al. 1997).

Sperm and egg chromatin exhibit extreme differences in methylationand structure. After breakdown of the pronuclear envelopes,the maternal and paternal chromosomes form a single metaphaseplate. However, despite extensive chromatin remodeling in thezygote, the unspecific germline differences are not completelyerased before the embryo cleaves into two cells. It seems plausibleto assume that the process of converting the complementary setsof maternal and paternal chromosomes into a specialized diploidsomatic genome may be regulated in a parent-specific mannerand occur in separate nuclear compartments. To test this hypothesis,we have used different in situ approaches demonstrating separationof chromatin according to parental origin in the fertilizedegg and the early diploid mouse embryo.

Materials and Methods

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Collection and Preparation of Mouse Preimplantation Embryos
Embryos for immunocytochemistry were derived from an intraspecificMus musculus (MMU) cross between (C57BL6 x C3H) F1, for simplicitytermed B6C3F1 mice. For fluorescence in situ hybridization (FISH)experiments, F1 embryos were derived from an interspecific crossbetween female laboratory mice, B6C3F1, and European wild mice,Mus spretus (MSP; strain SMZ).

Embryos were collected from superovulated mice according tostandard procedures (Hogan et al. 1994). Unfertilized oocytesfrom B6C3F1 mice were collected 18 h after human choriogonadotropin(hCG) injection. Fertilized one-cell embryos were prepared fromsuperovulated females mated with untreated males at 22 and 30h after hCG injection. Fertilization occurred $~$ 12 h (±1 h) after hCG treatment. Two-cell embryos were collected at34 and 44 h after hCG injection. Four-cell embryos were collected57 h after hCG. Eight-cell stages were flushed and collectedat 62 h, and morulae at 90 h after hCG treatment.

All embryos were released from the oviducts or uteri by insertinga 30-gauge needle into the infundibulum of the oviduct and injecting0.2 ml M2 flushing medium (Sigma Chemical Co.). One-cell embryoswere washed thoroughly in a drop of M2 medium containing 0.65mg/ml hyaluronidase and then several times in PBS to removeany maternal material. Two-cell embryos and more advanced stageswere washed in PBS only. The collected embryos were incubatedin a drop of hypotonic solution (50 mM KCl) for 2 h at 4°C.Each single embryo was transferred into a drop of ice-cold (4°C)fixative consisting of three parts methanol and one part glacialacetic acid, fixed for 40 min, and then transferred onto a cleanmicroscope slide. The embryo on the slide was covered with onedrop of a 1:1 mixture of methanol and acetic acid. After air-dryingof the fixative, the preparations were stored at 4°C forup to several weeks.

Preparation of Fibroblast Nuclei
Somatic cell nuclei were prepared from a primary fibroblastculture established from peritoneum of an adult F1 hybrid animal.Monolayer cells were grown in DME supplemented with 10% FBSand antibiotics. Cells were detached from culture flasks bygentle trypsinization, pelleted, and resuspended in 50 mM KCl.After a very short (<1 min) hypotonic treatment, cells werefixed overnight by adding four volumes of a 3:1 mixture of methanoland acetic acid. Slides were prepared using the conventionaldrop-splash technique.

BrdU Labeling of the Paternal Genome
Male B6C3F1 mice received an initial BrdU pulse by injectingi.p., 2 mg BrdU (in 200 µl PBS) and were then suppliedcontinuously with drinking water adjusted to pH 7.0 and containing0.5 mg/ml BrdU. Since BrdU is sensitive to daylight and luminescencefrom most lamps, the water bottles were wrapped with tin foiland the BrdU-containing water was changed at least once a week.BrdU is incorporated in place of thymidine into the replicatingDNA of mitotically dividing somatic and premeiotic cells. Thecycle time to produce mature spermatozoa from BrdU-labeled premeioticcells in mice is $~$ 35 d. After continuous BrdU feeding for atleast 5 wk, the BrdU-treated males were mated with superovulatedB6C3F1 females. Under the experimental conditions chosen, theBrdU was not toxic and did not induce recognizable developmentalabnormalities. Even after prolonged treatment (1 yr or longer),BrdU-treated males did not show obvious BrdU side effects andcould still be used for matings. Some pregnancies resultingfrom matings between BrdU-treated males and normal females wereallowed to go to term. The offspring produced and the littersize were normal.

Immunofluorescent Staining of BrdU-labeled DNA
BrdU-substituted DNA was visualized by a commercially availablemonoclonal anti-BrdU antibody (Boehringer Mannheim Corp.). Indouble-stranded DNA, the bromine atom is hidden in the phosphodiesterbackbone of the double helix and, therefore, not accessibleto antibody molecules. Since the anti-BrdU antibody only recognizesits chromosomal epitopes if the DNA is in the single-strandedform, the embryo preparations were denatured in 70% formamide,2x SSC for 1 min at 80°C and then dehydrated in an ice-coldethanol series (70, 85, and 100%). After brief air-drying, theslides were incubated at 37°C with mouse anti-BrdU antibody,diluted 1:50 with PBS, in a humidified incubator for 30 min.The slides were then washed in PBS three times for 10 min eachand incubated for 30 min with FITC-conjugated anti-mouse IgG(Dianova), appropriately diluted with PBS. After three furtherwashes with PBS, the preparations were counterstained with 1µg/ml 4',6-diamidino-2-phenylindole (DAPI) in 2x SSC for5 min. The slides were mounted in 90% glycerol, 0.1 M Tris-HCl,pH 8.0, and 2.3% 1,4-diazobicyclo-2,2,2-octane.

Fluorescence In Situ Hybridization
For FISH, the slides were treated with 100 µg/ml RNaseA in 2x SSC at 37°C for 60 min and with 0.01% pepsin in10 mM HCl at 37°C for 10 min, and then dehydrated in anethanol series (70, 85, and 100%). Slides were denatured at80°C in 70% formamide, 2x SSC, pH 7.0, and again dehydratedin an alcohol series. MSP genomic DNA was labeled by standardnick translation with biotin-16-dUTP and MMU genomic DNA withdigoxigenin-11-dUTP (Boehringer Mannheim Corp.). 10 ng/µleach of biotinylated MSP and digoxigenated MMU DNA were coprecipitatedwith 500 ng/µl salmon sperm carrier DNA, and redissolvedin 50% formamide, 10% dextran sulfate, 2x SSC. After 10 mindenaturation at 70°C, 30 µl of hybridization mixturewas applied to each slide and sealed under a coverslip. Slideswere left to hybridize in a moist chamber at 37°C for 1–3d. Slides were washed three times for 5 min in 50% formamide,2x SSC at 42°C, and once for 5 min in 0.1x SSC at 65°C,and blocked with 4x SSC, 3% BSA, and 0.1% Tween 20 at 37°Cfor 30 min. Biotinylated MSP DNA was detected by FITC-avidin(Vector Laboratories) and digoxigenated MMU DNA by Cy3-conjugatedantidigoxin antibody (Dianova). Chromosomes were counterstainedand mounted, as described above.

Digital Imaging Microscopy
Images were taken with a Zeiss epifluorescence microscope equippedwith a thermoelectronically cooled charge-coupled device camera(Photometrics CH250), which was controlled by an Apple Macintoshcomputer. Grayscale source images were captured separately withfilter sets for FITC, Cy3, and DAPI. Grayscale images were pseudocoloredand merged using ONCOR Image and Adobe Photoshop software. Itis worth emphasizing that, although a digital imaging systemwas used, all signals described here were clearly visible byeye through the microscope.

Results

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

Localization of BrdU-labeled Paternal DNA in Early Mouse Embryos
The germ-cell line in male mice was labeled with the halogenatedthymidine analogue BrdU, as described previously (Ito et al. 1988).This BrdU-substituted DNA was detected in embryos of the nextgeneration by anti-BrdU immunofluorescence staining and servedas a cytological marker for the paternal genome in interphasenuclei of the zygote and cleaving mouse embryo. Fig. 1 a showsa mouse egg upon fertilization. The condensed sperm nucleuscontained BrdU in both DNA strands of the paternal chromosomesand, therefore, was heavily labeled with the anti-BrdU antibody,whereas the activated female pronucleus was devoid of label.Decondensation of the sperm chromatin was followed by formationof the male pronucleus. Both the male and female pronuclei swelledand became apposed in the center of the zygote. The male pronucleusexhibited a nearly uniform punctate BrdU staining (Fig. 1 b).Since no localized (partial) labeling of the male pronucleuswas seen in >20 one-cell embryos analyzed at 10 and 18 hafter fertilization, we conclude that the entire male genomewas more or less uniformly substituted with BrdU. The smallerfemale pronuclei always remained BrdU negative, demonstratingthe specificity of the technique. Following a very short G₂phase of 1 h (Howlett 1986) and breakdown of the pronuclearenvelopes, the two chromosome sets remained completely separated,forming a single diploid nucleus (Fig. 1 c). Even in the absenceof colcemid, highly condensed metaphase chromosomes could beobserved at $~$ 20–22 h after fertilization (Fig. 1 d). Itis striking that the disruptive mitotic process did not leadto an intermingling of the two chromatin sets.

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Figure 1 Distribution of paternal chromatin in early mouse embryos. BrdU-treated male mice were mated with untreated females and the resulting embryos stained with FITC-conjugated anti-BrdU antibody (green). Nuclei and chromosomes were counterstained with DAPI (blue). a, Highly condensed sperm nucleus and fertilized egg (3). Numbers in parentheses indicate the number of embryos analyzed. b, Male and female pronuclei at 10 h after fertilization (20). The somewhat larger male pronucleus shows a nearly uniform BrdU staining, indicating that the entire sperm DNA is substituted with BrdU. c, After nuclear envelope breakdown the two chromosome sets form a single diploid nucleus (2). d, First metaphase at 20 h after fertilization (5). e, Two-cell embryo during G₁ phase at 22 h (>10). The second polar body remains completely BrdU negative. f, Two-cell embryo during G₂ phase at 32 h (>10). The male chromatin occupies approximately half of the nuclear volume. g, Four-cell embryo and second polar body at 45 h after fertilization (10). At this point, only half of the paternal chromosomes are still labeled with BrdU. h, 32-cell embryo at 78 h (>5). The one or two BrdU-positive sperm DNA strands per nucleus are consistent with random strand-segregation mechanisms. Bars, 10 µm.

Two-cell embryos in G₁ (>10) and G₂ phase (>10) were preparedat 22 and 32 h after fertilization. All paternal chromosomesin these two-cell embryos were still labeled with BrdU, butdue to the semiconservative DNA replication, in only one DNAstrand. In all two-cell embryos analyzed, the paternal chromosomeswere nonrandomly distributed throughout the entire nuclear volume.Usually each chromatin set occupied approximately one half ofthe nucleus (Fig. 1e and Fig. f), which is consistent with theview that paternal and maternal chromosomes remained completelyseparated. As expected, the second polar body, which was stillpresent on many embryo preparations (Fig. 1e and Fig. g), wasalways BrdU negative. Four-cell embryos were prepared afterthe second embryo cleavage at $~$ 45 h after fertilization. Thefact that after two replication cycles only half of the paternalchromosomes contained BrdU (sperm DNA strands) rendered topographicanalysis difficult. Nevertheless, most nuclei of four-cell embryosshowed a highly localized distribution of BrdU label withinthe nuclear area (Fig. 1 g), indicating that the parental genomeswere still separated at this point. Because of increasing lossof BrdU label with every successive replication cycle, the BrdUmethod is not suited for studying topological separation ofpaternal chromatin in more advanced preimplantation embryosor even in adult animals.

Segregation of the BrdU-labeled sperm chromosomes was followedup to the morula stage at 78 h after fertilization. Consistentwith the results of Ito et al. 1988, we found a random distributionof the 40 sperm DNA strands into different parts of the embryo.In well-spread preparations (Fig. 1 h), $~$ 50 distinct BrdU signalscould be seen on a 32-cell embryo. This somewhat too high number(there were only 40 BrdU-positive sperm DNA strands) may beexplained by the occurrence of sister chromatid exchanges duringpreceding interphases or be due to technical problems (splitimmunofluorescence signals).

Nonrandom Distribution of Paternal and Maternal Centromeres in Mouse Interspecific Hybrids
To rule out that the observed separation of parental genomesduring early embryogenesis was a result of BrdU incorporationinto sperm DNA, we used crosses between MMU and MSP, which divergedtwo to three million years ago (O'hUigin and Li 1992). Differencesin sequence and copy number of centromeric satellite DNAs (Matsuda and Chapman 1991)were used to identify maternal (MMU) and paternal (MSP) chromosomesin F1 hybrid embryos by FISH. By comparative hybridization ofdigoxigenated MMU genomic DNA and biotinylated MSP genomic DNA,the MMU (Fig. 2, red) and MSP centromeres (Fig. 2, green) werelabeled in different colors during both metaphase and interphase.However, since nonrepetitive MMU and MSP sequences show a polymorphismrate of only $~$ 1% (Takahashi and Ko 1993), it was not possibleto discriminate between maternal and paternal euchromatic chromosomearms by in situ methods (Fig. 2 a).

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Figure 2 Distribution of paternal and maternal centromeres in early mouse embryos derived from matings between (untreated) MSP males and MMU females. Biotinylated MSP genomic DNA and digoxigenated MMU genomic DNA were hybridized together and detected with FITC-avidin and Cy3-conjugated antidigoxin antibody. Chromosomes and nuclei were counterstained with DAPI (blue). a, Well-spread first metaphase of MMU x MSP hybrid embryo. The left image shows DAPI staining and the right image comparative FISH of the same spread. The maternal MMU centromeres exhibit red FISH signals. The paternal centromeres are stained in green. b, Two-cell F1 embryo (>10). Numbers in parentheses indicate the number of embryos analyzed. Maternal and paternal centromere complements remain separated and together occupy approximately half of the nucleus. c, Four-cell embryo showing genome separation and centromere clustering (10). Note the absence of green (paternal centromere) fluorescence in the polar body. d, Eight-cell embryo (5). Separation of the two centromere sets is seen in some, but not all, cells. Bars, 10 µm.

Consistent with our BrdU-labeling experiments, essentially all(>10) MMU x MSP two-cell embryos displayed a striking separationof maternal and paternal heterochromatin (Fig. 2 b). In addition,both the paternal and maternal centromeres were not evenly distributedthroughout the entire nuclear volume, but clustered togetherin one half of the nucleus. This orientation of centromeres,which was also seen in DAPI-stained preparations of normal MMUembryos (data not shown), was reminiscent of the Rabl polarizationof chromosomes (Rabl 1885). Distribution of centromeres at onecell pole and, by extrapolation, of (long-arm) telomeres atthe opposite cell pole may represent a passive relic of precedingmitosis. On the other hand, it may reflect an active chromosomearrangement to prevent intermingling of the two genomes. Centromereseparation and clustering were still visible in most nucleiof four-cell embryos (Fig. 2 c), but in <50% of nuclei ofeight-cell embryos (Fig. 2 d). The second polar body showedonly MMU centromere staining and, thus, served as a hybridizationcontrol. In more advanced 16–64-cell embryos, only 5–10%of cells demonstrated a nonrandom (localized) distribution ofthe two centromere sets (data not shown).

To learn whether genome separation is maintained in differentiatedcells, comparative genomic hybridization was performed on peritonealfibroblasts of an adult animal. Similar to the situation inadvanced embryo stages, relatively few (<10%) nuclei displayedclearly nonrandom heterochromatin staining patterns (Fig. 3a). One possible interpretation would be that in at least somesomatic cell types and/or cell-cycle stages the diploid chromosomecomplement may be separated in two haploid sets. Previous FISHstudies on human fibroblasts and HeLa cells suggested that homologouschromosomes and, by extrapolation, the paternal and maternalcomplements, may be positioned on opposite sites of the prometaphasechromosome rosette (Nagele et al. 1995). However, mouse interspecificfibroblasts showed a more or less random distribution of maternalMMU and paternal MSP chromosomes around the (pro)metaphase rosette(Fig. 3 b). Since clear separation of the two haploid sets wasnever observed in >50 prometaphases analyzed, the nonrandomdistribution of paternal and maternal centromeres in a proportionof interphase nuclei must arise through active chromosome (centromere)movements during interphase.

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Figure 3 Distribution of paternal (green) and maternal (red) centromeres in somatic cells of MMU x MSP hybrid animal. a, Peritoneal fibroblast nuclei (>500) displaying spatial separation of paternal and maternal heterochromatin blocks. Numbers in parentheses indicate the number of cells analyzed. Bar, 10 µm. b, Random distribution of MMU and MSP chromosomes around representative prometaphase rosettes (>50).

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

By two independent technical approaches, BrdU labeling of spermDNA and mouse interspecific hybrids, we have shown topologicalseparation of paternal and maternal chromatin in the early diploidmammalian embryo. Earlier autoradiographic experiments suggesteda nonrandom localization of radioactively labeled sperm DNAstrands in one- and two-cell mouse embryos (Odartchenko and Keneklis 1973).In a conceptually related study, also using BrdU to label thepaternal DNA, Ito et al. 1988 found random segregation of spermDNA strands in the developing mouse embryo. However, they didnot observe compartmentalization of parental chromatin. We feelthis may be due to differences in preparative techniques and/orto the small number of early preimplantation embryos analyzed.Thus, up to now the general belief was that the autoradiographicresults were experimental artifacts due to only partial labelingof the sperm genome and/or limited spatial resolution. Our studypresents the first comprehensive analysis of the higher-ordernuclear organization of parental chromatin during early mammaliandevelopment. Since we did not find regions of paternal pronucleifrom BrdU-treated males that remained completely unlabeled,we exclude the formal possibility that localization of BrdUlabel in later embryonic stages reflects partial labeling ofsperm DNA.

Topological separation of the parental genomes was preservedup to the four-cell embryo stage and then gradually disappearedor was no longer detectable with our in situ methods. A proportion(5–10%) of nuclei from more advanced embryos and evenof adult tissues still showed striking centromere separationin mouse interspecific hybrids. Although genome separation seemsto exist in at least some somatic cell types, it must be farless stable than in preimplantation embryos. It may be difficultto observe, because it is transient and/or modulated by thecell cycle. Since separation of haploid chromosome sets wasnot seen in prometaphase rosettes, nonrandom distribution ofpaternal and maternal interphase heterochromatin does not passivelyreflect mitotic chromosome arrangement. However, at presentwe cannot rule out that compartmentalization of MMU and MSPchromosomes in somatic cells may be a secondary (hybrid) effect.Association between heterochromatic blocks may be mediated bysimilar chemical properties of the chromatin in these chromosomeregions, such as the high concentration of simple repeats. Pairingof regions with identical or closely related repeat DNAs maybe preferred over those between more diverged regions (Haaf et al. 1986),explaining the formation of two separate heterochromatic compartmentsin mouse interspecific nuclei.

Accumulating experimental evidence suggests that higher-ordernuclear organization may influence both normal developmentaland pathological cellular processes and, hence, deserves tobe studied in greater detail. Nuclear architecture is thoughtto provide a structural framework that may affect the accessibilityof chromatin to regulatory factors and, thus, may serve an essentialrole in the regulation of gene expression beyond that at thesingle-gene level (Manuelidis and Borden 1988; Haaf and Schmid 1991).In situ methods are extremely powerful tools for elucidatingthe relationship between nuclear structure and function. Ourexperiments clearly demonstrate that paternal and maternal chromatinoccupy separate nuclear entities at the time of preimplantationdevelopment when epigenetic chromatin remodelling (Mayer et al. 2000)and programming of the appropriate patterns of parent-specificdevelopmental gene expression occur (Fundele and Surani 1994).We argue in favor of the notion that genome separation duringearly mammalian development is functionally important, ratherthan a passive consequence of the different histories of spermand egg chromation before fertilization. In addition, genomeseparation may serve a functional role in at least some differentiatedcell types. While highly speculative, it is interesting to considerthe possibility that disturbances in genome separation are notcompatible with normal embryogenesis and are an important reasonfor early embryo loss, i.e., after in vitro fertilization, parthenogenesis,or mammalian cloning.

Acknowledgments

We thank Annie Orth and Francois Bonhomme (University of MontpellierII) for providing M. spretus mice.

Submitted: 9 November 1999

Revised: 6 January 2000

Accepted: 7 January 2000

The authors dedicate this paper to the memory of Wolfgang Mayerwho died on August 19, 1999.

Abbreviations used in this paper: BrdU, 5-bromodeoxyuridine;DAPI, 4',6-diamidino-2-phenylindole; FISH, fluorescence in situhybridization; hCG, human choriogonadotropin; MMU, Mus musculus;MSP, Mus spretus.

References

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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