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用于细胞质抗原、溴脱氧尿苷和DNA三重标记的固定和变性方法的选择。应用于骨髓浆细胞。

Choice of fixation and denaturation for the triple labelling of intra-cytoplasmic antigen, bromodeoxyuridine and DNA. Application to bone marrow plasma cells.

作者信息

Ffrench M, Morel F, Souchier C, Benchaib M, Catallo R, Bryon P A

机构信息

Laboratoire de Cytologie Analytique, Faculté de Médecine, Lyon, France.

出版信息

Histochemistry. 1994 Jun;101(5):385-90. doi: 10.1007/BF00269001.

DOI:10.1007/BF00269001
PMID:7523339
Abstract

A triple staining method of intra-cytoplasmic antigen, bromodeoxyuridine (BrdU), and DNA for fluorescence image analysis is described. Several kinds of fixation and DNA denaturation methods were tested to obtain a technique suitable for heterogeneous tissues. The model chosen was the analysis of plasma cells in bone marrow. The fluorochromes used were fluorescein isothiocyanate (FITC) for intra-cytoplasmic antigens (light chain immunoglobulins), aminomethylcoumarin acetic acid (AMCA) for BrdU, and propidium iodide (PI) for DNA. The quality of the staining was analysed according to: (1) cell morphology with a good preservation of the chromatin structure, (2) intensity of light chains and of BrdU labelling, and (3) the quality of DNA staining judged from a DNA histogram. For most of the analysed tissues, fixation with methanol followed by 0.5% paraformaldehyde and denaturation by an NaOH concentration adapted to the tissue gave good results. However, in our model fixation by methanol, followed by methanol/acetic acid and denaturation of DNA by 0.03 N NaOH was the solely satisfactory technique. A good correlation (P < 0.001) was found with the plasma cell BrdU labelling index obtained with our reference immuno-enzymatic technique. Quantification of DNA content showed a satisfactory G1 peak coefficient of variation (CV) in diploid cells and a 4C to 2C ratio equal to 2. With this technique, the nuclear and cytoplasmic structures of both myeloid cells and plasma cells were well preserved, while their sensitivity to DNA denaturation was quite different.

摘要

本文描述了一种用于荧光图像分析的胞浆内抗原、溴脱氧尿苷(BrdU)和DNA的三重染色方法。测试了几种固定和DNA变性方法,以获得适用于异质性组织的技术。所选模型为骨髓浆细胞分析。所用荧光染料为:异硫氰酸荧光素(FITC)用于胞浆内抗原(轻链免疫球蛋白),氨基甲基香豆素乙酸(AMCA)用于BrdU,碘化丙啶(PI)用于DNA。根据以下方面分析染色质量:(1)细胞形态,染色质结构保存良好;(2)轻链和BrdU标记的强度;(3)从DNA直方图判断的DNA染色质量。对于大多数分析的组织,先用甲醇固定,再用0.5%多聚甲醛固定,并用适合该组织的NaOH浓度进行变性,可得到良好结果。然而,在我们的模型中,先用甲醇固定,再用甲醇/乙酸固定,并用0.03 N NaOH对DNA进行变性,是唯一令人满意的技术。与我们的参考免疫酶技术获得的浆细胞BrdU标记指数有良好的相关性(P < 0.001)。DNA含量的定量分析显示,二倍体细胞中G1峰变异系数(CV)令人满意,4C与2C的比值等于2。采用该技术,髓细胞和浆细胞的核结构和胞质结构均保存良好,而它们对DNA变性的敏感性差异很大。

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