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- W2034939094 abstract "OBJECTIVE: Our purpose was to compare murine embryo development after pronuclear microinjection of a gene construct, followed by trophectoderm biopsy at the blastocyst state, with development after a single micromanipulation, and with cultured controls. STUDY DESIGN: α-Myosin heavy-chain gene sequence was microinjected into the murine embryo pronucleus and cultured to blastocyst. After trophectoderm biopsy the embryos were allowed to reexpand. Reexpanded embryos were transferred to pseudopregnant females; implantation and live birth rates were recorded. In this study group the rates were compared with three control groups of embryos simultaneously cultured after (1) pronuclear microinjection only, (2) trophectoderm biopsy only, and (3) nonmicromanipulated, culture only. RESULTS: A total of 1222 embryos were divided among the four groups. In the study group 472 embryos underwent pronuclear microinjection and trophectoderm biopsy. Of these, 203 (43%) reached the blastocyst stage and underwent biopsy; 183 (38.8%) reexpanded after biopsy. Of 275 pronuclear microinjected only (control 1) embryos, 113 (41.1%) reached the blastocyst stage. Of 336 embryos 148 (44.0%) reached the blastocyst stage and underwent trophectoderm biopsy only (control 2); 129 (39.2%) survived biopsy. The cultured only group (control 3) consisted of 139 pronuclear embryos; 67 (48.2%) developed to the blastocyst stage. CONCLUSIONS: Murine embryos can survive two micromanipulations, pronuclear microinjection followed by trophectoderm microbiopsy. Although there is minimal effect of these procedures on embryonic development in vitro, the live birth rate is tenuous. (AM J OBSTET GYNECOL 1994;170:1199-203.)" @default.
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- W2034939094 date "1987-01-01" @default.
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- W2034939094 title "A micromanipulation system controlled by personal computer for microsurgery on fertilized ova and embryos" @default.
- W2034939094 doi "https://doi.org/10.1016/0093-691x(87)90175-0" @default.
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