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利用DNA和核蛋白的同步流式细胞术测量对细胞动力学反应进行定量分析。

Quantitation of cell kinetic responses using simultaneous flow cytometric measurements of DNA and nuclear protein.

作者信息

Pollack A, Moulis H, Block N L, Irvin G L

出版信息

Cytometry. 1984 Sep;5(5):473-81. doi: 10.1002/cyto.990050507.

DOI:10.1002/cyto.990050507
PMID:6489061
Abstract

A rapid procedure was developed for the simultaneous flow cytometric analysis of nuclear protein using fluorescein isothiocyanate, and DNA using propidium iodide in isolated nuclei. The staining procedure did not involve centrifugation and was easily adapted to the staining of human peripheral blood lymphocytes stimulated with phytohemagglutinin, EL4 murine lymphoid tumor cells in suspension culture, and R3327-G rat prostatic adenocarcinoma solid tumor specimens. Histograms of unstimulated and PHA-stimulated HPBL perturbed by actinomycin D, hydroxyurea, 3H-TdR, colcemid, or hydroxyurea + colcemid showed that 1) resting, noncycling G1 (G1Q) cells are distinguished from late G1 (G1AB) cells, 2) early G2 (G2A) cells are distinguished from late G2 (G2B) cells, and 3) mitotic cells are distinguished from G2 cells. Treatment with hydroxyurea resulted in a build-up of cells having high nuclear protein content and 2C DNA content (G1AB), while incubation with 3H-TdR caused an increase in the number of cells with high nuclear protein content and 4C DNA content (G2B). Colcemid-blocked mitotic cells were identified as having low nuclear protein content (lower than G2A nuclei) and 4C DNA content. The nuclear DNA/protein histograms of untreated and colcemid-treated log-phase EL4 cells provided information concerning G1A, G1B, S, G2A, G2B, and M. The method was also used to quantitate the response of androgen-sensitive rat prostatic R3327-G tumors to androgen deprivation following castration. Sample preparation and staining for correlated nuclear DNA/protein measurements takes approximately the same amount of time as for single parameter nuclear DNA measurements.

摘要

开发了一种快速程序,用于在分离的细胞核中同时使用异硫氰酸荧光素进行核蛋白的流式细胞术分析,并使用碘化丙啶进行DNA分析。染色程序不涉及离心,并且很容易适用于用植物血凝素刺激的人外周血淋巴细胞、悬浮培养的EL4鼠淋巴瘤细胞以及R3327-G大鼠前列腺腺癌实体瘤标本的染色。未刺激的和经植物血凝素刺激的人外周血淋巴细胞受放线菌素D、羟基脲、3H-胸腺嘧啶核苷、秋水仙酰胺或羟基脲+秋水仙酰胺干扰后的直方图显示:1)静止的、非循环的G1(G1Q)细胞与晚期G1(G1AB)细胞有区别;2)早期G2(G2A)细胞与晚期G2(G2B)细胞有区别;3)有丝分裂细胞与G2细胞有区别。用羟基脲处理导致具有高核蛋白含量和2C DNA含量(G1AB)的细胞积累,而与3H-胸腺嘧啶核苷孵育导致具有高核蛋白含量和4C DNA含量(G2B)的细胞数量增加。秋水仙酰胺阻断的有丝分裂细胞被鉴定为具有低核蛋白含量(低于G2A细胞核)和4C DNA含量。未处理的和经秋水仙酰胺处理的对数期EL4细胞的核DNA/蛋白直方图提供了有关G1A、G1B、S、G2A、G2B和M期的信息。该方法还用于定量雄激素敏感的大鼠前列腺R3327-G肿瘤在去势后对雄激素剥夺的反应。用于相关核DNA/蛋白测量的样品制备和染色所需时间与单参数核DNA测量大致相同。

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Nuclear protein as a prognostic factor of growth activity in prostatic adenocarcinoma.核蛋白作为前列腺腺癌生长活性的预后因素。
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2
Cytotoxic properties of a new synthetic demethylpodophyllotoxin derivative, BN 58705, against human tumor cell lines.一种新型合成去甲基鬼臼毒素衍生物BN 58705对人肿瘤细胞系的细胞毒性特性
Cancer Chemother Pharmacol. 1993;32(4):293-300. doi: 10.1007/BF00686175.
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Flow cytometric DNA histograms and type of growth.流式细胞术DNA直方图与生长类型
J Cancer Res Clin Oncol. 1988;114(6):559-64. doi: 10.1007/BF00398177.
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Prediction of thioguanine-induced cytotoxicity by dual-parameter flow cytometric analysis.
Cancer Chemother Pharmacol. 1989;24(5):291-4. doi: 10.1007/BF00304760.
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Flow cytometric analysis of the mechanism of methylmercury cytotoxicity.甲基汞细胞毒性机制的流式细胞术分析
Am J Pathol. 1990 Nov;137(5):1187-98.