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肝细胞增殖研究的分析方法。

Analytical methods for the study of liver cell proliferation.

作者信息

Gerlyng P, Stokke T, Huitfeldt H S, Stenersen T, Danielsen H E, Grotmol T, Seglen P O

机构信息

Department of Tissue Culture, Norwegian Radium Hospital, Oslo.

出版信息

Cytometry. 1992;13(4):404-15. doi: 10.1002/cyto.990130411.

Abstract

Various cytometric methods for analysis of regenerating rat liver growth (DNA ploidy distributions, binucleation, and DNA synthesis by in vivo BrdUrd incorporation) were evaluated. The overall hepatocellular growth rate (labeling index), the binucleation rate, and separate indices for mononuclear and binuclear cells could be measured simply by microscope counting of collagenase-isolated hepatocytes immunostained for BrdUrd. Flow cytometry of cells stained for BrdUrd and DNA provided labeling indices for the various hepatocellular DNA ploidy classes as well as for nonparenchymal cells (identified by their size-dependent light scatter), but could not distinguish between mononuclear and binuclear hepatocytes. Image cytometry, using fluorescence or Feulgen staining, was inferior to flow cytometry in terms of speed and DNA resolution, but allowed a complete analysis of all hepatocellular DNA ploidy and nuclearity classes. It may therefore be the method of choice, particularly for analysis of liver cell cultures from which single cells are not easily obtained. Fluorescence staining would seem to be preferable to Feulgen staining, since the latter could not be used simultaneously with BrdUrd staining and therefore required a two-step analysis. A non-immunological method, based on the ability of incorporated BrdUrd to quench DNA staining by a Hoechst dye, could only be applied to isolated nuclei, thus giving no information about binucleation. The latter method may be useful for analysis of tumors which are difficult to dissociate to intact whole cells.

摘要

评估了多种用于分析再生大鼠肝脏生长的细胞计数方法(DNA倍体分布、双核化以及通过体内掺入溴脱氧尿苷进行DNA合成)。通过对经胶原酶分离并用溴脱氧尿苷免疫染色的肝细胞进行显微镜计数,可简单地测量总体肝细胞生长速率(标记指数)、双核化速率以及单核和双核细胞的单独指数。对经溴脱氧尿苷和DNA染色的细胞进行流式细胞术分析,可提供各种肝细胞DNA倍体类别的标记指数以及非实质细胞(通过其大小依赖性光散射识别)的标记指数,但无法区分单核和双核肝细胞。使用荧光或福尔根染色的图像细胞术在速度和DNA分辨率方面不如流式细胞术,但能对所有肝细胞DNA倍体和核型类别进行完整分析。因此,它可能是首选方法,尤其适用于分析不易获得单细胞的肝细胞培养物。荧光染色似乎比福尔根染色更可取,因为后者不能与溴脱氧尿苷染色同时使用,因此需要两步分析。一种基于掺入的溴脱氧尿苷淬灭Hoechst染料对DNA染色能力的非免疫方法只能应用于分离的细胞核,因此无法提供有关双核化的信息。后一种方法可能对难以解离为完整全细胞的肿瘤分析有用。

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