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[小鼠细胞计数DNA含量的器官间差异:染色方法的关系]

[Inter-organ differences of the cytometric DNA content in mice: relation of the staining method].

作者信息

Vago P, Aboudkhil S, Aguilar V, Bureau J P

机构信息

Laboratoire de Biologie Cellulaire et d'Immunogénétique, Faculté de Médecine, Nîmes.

出版信息

C R Seances Soc Biol Fil. 1988;182(5):494-500.

PMID:2977968
Abstract

With one step DNA staining methods including cell membrane lysis and RNase treatment, we regularly observed a higher fluorescence emission in liver nuclei compared to bone marrow nuclei in C57BL/6 mice. Therefore this study was conducted in order to emphasize such a phenomenon in other organs and to assess if higher fluorescence emission was related to higher DNA content or staining procedure failure. Liver, bone marrow and testis were removed from Swiss, BDF and C57BL/6 mice. The following samples were prepared: 1) liver cells with TRBC (TRBC = Trout Red Blood Cells = internal standards), 2) bone marrow cells with TRBC, 3) testis cells with TRBC and 4) mixtures of liver, bone marrow and testis cells. The staining procedures were: A) one step pH 10 procedure described by Vindelov (Virchows Arch. B. Cell Path., 1977, 24, 227-242), B) same procedure with twice RNase concentration, C) first method with twice NP 40 concentration and D) three steps procedure including Trypsin and Spermine treatment (Vindelov et al., Cytometry, 1983, 3, 323-327). In protocols A, B and C, "Diploid cells/TRBC" ratio differed significantly between liver, bone marrow and testis nuclei. Moreover, 3 distinct populations of diploid cells were present in samples 4. In protocol D, "Diploid cells/TRBC" ratio were identical between liver, bone marrow and testis nuclei. In samples 4, only 1 population of diploid cells has been observed. This study shows that DNA stabilization by polyamine and protein degradation by protease could act on Propidium Iodide fixation and/or fluorescence emission, with significant differences according to the origin of the cells.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

采用包括细胞膜裂解和核糖核酸酶处理在内的一步DNA染色方法,我们经常观察到,在C57BL/6小鼠中,肝细胞核的荧光发射比骨髓细胞核更高。因此,开展本研究是为了在其他器官中强调这种现象,并评估较高的荧光发射是否与较高的DNA含量或染色程序失败有关。从瑞士小鼠、BDF小鼠和C57BL/6小鼠身上取出肝脏、骨髓和睾丸。制备了以下样本:1)含有TRBC的肝细胞(TRBC = 鲑鱼红细胞 = 内标),2)含有TRBC的骨髓细胞,3)含有TRBC的睾丸细胞,以及4)肝脏、骨髓和睾丸细胞的混合物。染色程序如下:A)Vindelov描述的一步pH 10程序(《Virchows Arch. B. Cell Path.》,1977年,第24卷,第227 - 242页),B)核糖核酸酶浓度加倍的相同程序,C)NP 40浓度加倍的第一种方法,以及D)包括胰蛋白酶和精胺处理的三步程序(Vindelov等人,《Cytometry》,1983年,第3卷,第323 - 327页)。在方案A、B和C中,肝细胞核、骨髓细胞核和睾丸细胞核之间的“二倍体细胞/TRBC”比率存在显著差异。此外,样本4中存在3个不同的二倍体细胞群体。在方案D中,肝细胞核、骨髓细胞核和睾丸细胞核之间的“二倍体细胞/TRBC”比率相同。在样本4中,仅观察到1个二倍体细胞群体。本研究表明,多胺对DNA的稳定作用和蛋白酶对蛋白质的降解作用可能影响碘化丙啶固定和/或荧光发射,根据细胞来源不同存在显著差异。(摘要截选至250词)

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