BRIEF REPORT |
Topology of Chromosomes 18 and X in Human Blastomeres from 3- to 4-Day-old Embryos
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Center of Reproductive Genetics, Institute of Biology and Medical Genetics, Charles University, 2nd School of Medicine, University Hospital Motol, Prague, Czech Republic (JD,MM); Società Italiana Studi di Medicina della Riproduzione, Bologna, Italy (MCM,LG); and Department of Genetics and Microbiology, Charles University, Faculty of Science, Prague, Czech Republic (RK)
Correspondence to: Milan Macek Sr., Institute of Biology and Medical Genetics, University Hospital Motol, V Úvalu 84, Prague 5 CZ-150 06, Czech Republic. E-mail: pavel.roubic{at}lfmotol.cuni.cz
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Summary |
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(J Histochem Cytochem 53:273276, 2005)
Key Words: chromosome localization FISH chromosome 18 chromosome X human blastomeres
HUMAN INTERPHASE chromosomes occupy discrete territories within the nucleus. Chromosomes with a high gene density content (e.g., chromosome 19) are localized in the interior of the nucleus, whereas chromosomes with a comparatively lower gene content (e.g., chromosomes 18 and X) are localized peripherally (Cremer et al. 2001; Weierich et al. 2003
; Kreth et al. 2004
). Inactivated X chromosome is also localized in the nuclear periphery as a "sex chromatin body" (Comings 1967
). Thus far, performed studies of human chromosomal localization within nuclei utilized lymphocytes, fibroblasts, and amniocytes (Cremer et al. 2001
).
The aim of this study was to determine whether human chromosomes 18 and X, localized at the nuclear periphery in later periods of development (Cremer et al. 2001), follow a similar pattern also in blastomeres from 3- to 4-day-old human embryos generated by in vitro fertilization (IVF).
Preimplantation genetic screening (PGS) of aneuploidies of chromosomes 13, 16, 18, 21, 22, X, and Y was performed within 32 IVF cycles in 28 infertile couples. Four of the couples had two successive IVF cycles. Informed consent was obtained from all studied subjects, and the study was approved by the local ethics board for all acknowledged research projects.
All embryos from 26 IVF cycles were analyzed. Mean age of the women at the time of oocyte retrieval was 32.2 years (ranging between 25 and 40 years). Respective indications for IVF included advanced maternal age (7/26), repeated failure of IVF (8/26), repeated miscarriages (3/26), previous pregnancy with an aneuploid fetus (1/26), infertility related to immunological factors (11/26), mosaic forms of Turner syndrome (2/26), previous cytostatic therapy (3/26), and gender selection in a hemophilia A carrier (1/26). Partners' oligozoospermia was found in 12/26, while in 2/26 partners' sperm, concentration was <1 million/ml.
In total, 204 blastomeres were examined. However, only 110 blastomeres (53.9%) without multinucleation, fragmentation of nuclei, and/or damage of fluorescence in situ hybridization (FISH) signals were selected for further analyses. Blastomeres with nullisomy of chromosomes 18 and/or X were excluded from the study.
Blastomere biopsy was performed on days 3 to 4 according to their total number in analyzed embryos. Blastomeres were washed in a hypotonic solution (1% sodium citrate, 0.6% BSA), followed by air-drying fixation (methanol and acetic acid, 3:1 ratio). Two-round FISH (Magli et al. 2001) utilizing the Vysis MultiVysion PB probe panel (Abbott Laboratories; Abbott Park, IL) with fluorescent probes for chromosomes 13, 16, 18, 21, and 22 and Vysis CEP X + CEP Y Alpha (Abbott) sets were employed. Axioplan 2 MOT microscope (Carl Zeiss, Oberkochen, Germany) with single, double, and quadruple bandpass filters and x63 Plan-Apochromat objective were used. Images were captured using Axiocam MRm (Zeiss) camera and either Axiovision (Zeiss) or ISIS (Metasystems; Altlussheim, Germany) software. Images were exported as bitmap files and analyzed by ImageJ 1.32 (National Institutes of Health, available on the internet at http://rsb.info.nih.gov/ij/) software. Prevalence of detected aneuploidies is documented in Tables 1 and 2.
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The relative signal distance (RD) was calculated by the equation: RD = Rs/R, where "Rs" is distance of the signal center from the center of the nucleus and "R" is the radius of the nucleus (Figures 1A and 1B). The RD measurements yielded values between 0 and almost 1.0, because completely peripherally located signals did not achieve the value of 1.0. This is because their center is always separated from the nuclear border edge by the distance equaling the radius of the signal itself (Figure 1B). In total, we measured the localization of 386 fluorescent signals.
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Relative distances (RD) of 386 measured signals of chromosomes 18 and X and of chromosome X in cells with one or two chromosomes X and in cells with different chromosomal aneuploidies (Table 3) were compared.
Statistically significant differences were found only between distributions expected from the 3D sphere model and observed distributions of RD values for chromosome 18 in all blastomeres (p=0.0011) and in aneuploid cells only (p=0.0013) (Table 3). In euploid cells, such a difference was not significant (p=0.53). These data strongly suggest peripheral localization of chromosome 18 within a sample of blastomeres, either aneuploid only and/or where euploid and aneuploid cells were studied together. This finding is in agreement with the study of McKenzie et al. (2004).
If further studies also provide evidence of the impact of chromosomal aneuploidy on early peripheral localization of chromosome 18 within the blastomere nucleus, a better understanding of the pathogenesis of early development disorders and mutual chromosome interactions in this process might be gained.
Absence of statistically significant shift to the periphery of chromosome X in both euploid and aneuploid female blastomeres did not prove peripheral localization, and thus genetic inactivation, of chromosome X in 3- to 4-day-old female embryos.
Our preliminary results will be confirmed by our further studies using higher numbers of blastomeres, stratified according to the respective PGS indication, parental age, and in relation to different types of autosomal and heterochromosomal aneuploidies. The most exact evaluation of chromosome topology can be obtained only by 3D FISH methods (Cremer et al. 2001) that so far are not feasible for PGS performed in human blastomeres.
Obtained results stress the importance of further studies of chromosome topology to verify the possible role of aneuploidy on particular chromosome localization. Such studies will also elucidate respective gene expression, including the onset of early X chromosome inactivation in 3- to 4-day-old female IVF embryos. The likely practical outcome could be improved selection of embryos for transfer after preimplantation prenatal genetic diagnosis.
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Acknowledgments |
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We would like to thank Prof Milan Macek Jr DSc for critical review of this manuscript.
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Footnotes |
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Received for publication June 10, 2004; accepted November 12, 2004
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Literature Cited |
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Comings DE (1967) The duration of replication of the inactive X chromosome in humans based on the persistence of the heterochromatic sex chromatin body during DNA synthesis. Cytogenetics 6:2037[Medline]
Cremer M, von Hase J, Volm T, Brero A, Kreth G, Walter J, Fischer C, et al. (2001) Non-random radial higher-order chromatin arrangements in nuclei of diploid human cells. Chromosome Res 9:541567[CrossRef][Medline]
Kreth G, Finsterle J, von Hase J, Cremer M, Cremer C (2004) Radial arrangement of chromosome territories in human cell nuclei: a computer model approach based on gene density indicates a probabilistic global positioning code. Biophys J 86:28032812
Magli MC, Sandalinas M, Escudero T, Morrison L, Ferraretti AP, Gianaroli L, Munne S (2001) Double locus analysis of chromosome 21 for preimplantation genetic diagnosis of aneuploidy. Prenat Diagn 21:10801085[CrossRef][Medline]
McKenzie LJ, Carson SA, Marcelli S, Rooney E, Cisneros P, Torskey S, Buster J, et al. (2004) Nuclear chromosomal localization in human preimplantation embryos: correlation with aneuploidy and embryo morphology. Hum Reprod 19:22312237
Weierich C, Brero A, Stein S, von Hase J, Cremer C, Cremer T, Solovei I (2003) Three-dimensional arrangements of centromeres and telomeres in nuclei of human and murine lymphocytes. Chromosome Res 11:485502[CrossRef][Medline]