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根据精子发生过程中的DNA和线粒体变化对小鼠睾丸细胞进行分选。

Mouse testis cell sorting according to DNA and mitochondrial changes during spermatogenesis.

作者信息

Petit J M, Ratinaud M H, Cordelli E, Spanò M, Julien R

机构信息

Institut de Biotechnologie, Faculté des Sciences, Limoges, France.

出版信息

Cytometry. 1995 Apr 1;19(4):304-12. doi: 10.1002/cyto.990190404.

Abstract

Flow cytometry can measure variations in DNA content and chromatin structure as well as dramatic changes in the mitochondria of germ cells during maturation from spermatogonia to elongated spermatids. Using 10-N nonyl acridine orange (NAO), an inner mitochondrial membrane dye, it is easy to follow mitochondria rearrangements. Mouse testis cells stained with the DNA fluorescent probe propidium iodide (PI) and analyzed by flow cytometry can be discriminated on the basis of their ploidy levels into five main regions corresponding to elongated spermatids, round spermatids, diploid, S-phase, and tetraploid cells. The simultaneous use of PI and NAO demonstrated the presence of cells having low and high mitochondrial content in the haploid, diploid, and tetraploid compartments. Eleven sorting windows were selected from the bivariate analysis (PI/NAO) and the corresponding cells were identified by microscopic observation. Cells were also discriminated by two parameter analysis of DNA content vs. cell diameter. The definition of seven different regions allowed us to determine NAO or rhodamine 123 (Rh 123) uptakes in each compartment. We observed that the ratio (Rh 123/NAO) dramatically changed according to the progression of cell differentiation which occurs during spermatogenesis.

摘要

流式细胞术可以测量从精原细胞到延长型精子细胞成熟过程中生殖细胞的DNA含量、染色质结构变化以及线粒体的显著改变。使用10-N壬基吖啶橙(NAO)这种线粒体内膜染料,很容易追踪线粒体的重排。用DNA荧光探针碘化丙啶(PI)染色并通过流式细胞术分析的小鼠睾丸细胞,可以根据其倍性水平分为五个主要区域,分别对应延长型精子细胞、圆形精子细胞、二倍体细胞、S期细胞和四倍体细胞。同时使用PI和NAO显示,在单倍体、二倍体和四倍体区室中存在线粒体含量低和高的细胞。从双变量分析(PI/NAO)中选择了11个分选窗口,并通过显微镜观察鉴定了相应的细胞。细胞也通过DNA含量与细胞直径的双参数分析进行区分。定义七个不同区域使我们能够确定每个区室中NAO或罗丹明123(Rh 123)的摄取情况。我们观察到,(Rh 123/NAO)比值随着精子发生过程中细胞分化的进展而显著变化。

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