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通过胞质分裂阻断微核试验预测肿瘤放射敏感性

Tumor radiosensitivity prediction by the cytokinesis-block micronucleus assay.

作者信息

Shibamoto Y, Streffer C, Fuhrmann C, Budach V

机构信息

Institute of Medical Radiation Biology, University of Essen, Germany.

出版信息

Radiat Res. 1991 Dec;128(3):293-300.

PMID:1961926
Abstract

An in vivo to in vitro cytokinesis-block micronucleus assay technique using cytochalasin B (Cyt-B) was established in xenografted human and murine tumors, and the correlation between radiosensitivity measured by this assay and that measured by a colony-forming assay was investigated. Tumors were irradiated in situ, excised immediately, and disaggregated to single cells that were plated for the micronucleus and colony-forming assays. Some of the tumor cells were irradiated in vitro rather than in vivo. For the micronucleus assay, Cyt-B (0.5-3 micrograms/ml) was added to dishes soon after plating or in vitro irradiation and the cells were subsequently fixed and stained at intervals (12-144 h). The micronucleus frequency in binucleate cells was evaluated under conditions of maximum yield of the binucleate cells. The micronucleus frequency after irradiation was quite variable depending on the tumor type and the average number of micronuclei per single binucleate cell after 4 Gy ranged from 0.2 to 1.4. The results of in vitro irradiation were not significantly different from those of in vivo irradiation for all tumors. A good correlation was found between the radiosensitivity determined by the micronucleus assay and that found with the colony-forming assay in six human tumors (r = 0.94 approximately 0.98) but not in four murine tumors because of one exceptional tumor. When this tumor was excluded, a correlation was also found for the remaining nine tumors (r = 0.62 approximately 0.96). These results indicated that the cytokinesis-block micronucleus assay has some promise as a rapid predictive assay of radiosensitivity.

摘要

在异种移植的人源和鼠源肿瘤中建立了一种使用细胞松弛素B(Cyt - B)的体内到体外胞质分裂阻断微核试验技术,并研究了该试验所测放射敏感性与集落形成试验所测放射敏感性之间的相关性。肿瘤在原位接受照射,然后立即切除并解离成单细胞,接种用于微核试验和集落形成试验。部分肿瘤细胞是在体外而非体内接受照射。对于微核试验,在接种后或体外照射后不久向培养皿中加入Cyt - B(0.5 - 3微克/毫升),随后在不同时间间隔(12 - 144小时)对细胞进行固定和染色。在双核细胞产量最高的条件下评估双核细胞中的微核频率。照射后的微核频率因肿瘤类型而异,4 Gy照射后每个单核双核细胞的微核平均数在0.2至1.4之间。对于所有肿瘤,体外照射的结果与体内照射的结果无显著差异。在6种人类肿瘤中,微核试验所测放射敏感性与集落形成试验所测放射敏感性之间存在良好的相关性(r = 0.94至0.98),但在4种鼠源肿瘤中未发现相关性,因为有一个特殊肿瘤。排除该肿瘤后,其余9种肿瘤也发现了相关性(r = 约0.62至0.96)。这些结果表明,胞质分裂阻断微核试验作为一种快速预测放射敏感性的试验具有一定前景。

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