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A reliable, noninvasive technique for spindle imaging and enucleation of mammalian oocytes.

作者信息

Liu L, Oldenbourg R, Trimarchi J R, Keefe D L

机构信息

[1] Department of Ob/Gyn, Women and Infants Hospital, Brown University, Providence, RI 02905.[2] Marine Biological Laboratory, Woods Hole, MA 02543, USA.

出版信息

Nat Biotechnol. 2000 Feb;18(2):223-5. doi: 10.1038/72692.

DOI:10.1038/72692
PMID:10657133
Abstract

Factors affecting the efficiency of animal cloning remain to be elucidated. Enucleation of recipient oocytes is a critical step in cloning procedures and typically is performed by aspirating a portion of the cytoplasm underlying the first polar body. Enucleation is evaluated using epifluorescence after Hoechst staining for DNA, which may disrupt functions of the cytoplast, especially mitochondria. Mitochondrial DNA in Dolly and other cloned sheep has been shown to derive exclusively from recipient oocytes. Not only might evaluation of the aspirated karyoplast portion inadequately reflect the state of the cytoplast, it is also time consuming. Here we report a reliable, noninvasive technique for spindle imaging and enucleation of oocytes using a new microscope, the Pol-Scope. The efficiency of enucleation was 100%, and only 5.5% of the oocytes' mitochondria entered the karyoplast upon Pol-Scope-directed removal of the spindle. Moreover, Pol-Scope imaging of spindles and micromanipulation did not compromise the developmental competence of reconstituted oocytes and cytoplasts.

摘要

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