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用氚标记胸腺嘧啶核苷对实体组织进行体外标记,用于自显影检测S期细胞核。

In vitro labeling of solid tissues with tritiated thymidine for autoradiographic detection of S-phase nuclei.

作者信息

Meyer J S, Connor R E

出版信息

Stain Technol. 1977 Jul;52(4):185-95. doi: 10.3109/10520297709116774.

DOI:10.3109/10520297709116774
PMID:143737
Abstract

In vitro measurement of the thymidine labeling index (TLI) of solid tissues requires hyperbaric oxygenation and is potentiated by blockade of thymidylate synthetase by 5-fluoro-2'-deoxyuridine (FUdR) to favor uptake of tritiated thymidine (3H-TdR). Hyperbaric oxygenation can be achieved in a simple system through injection of oxygen into rubber-stoppered test tubes. Incubations are carried out in Hanks' balanced salt solution in a shaker bath at 37 C for 2 hours; an FUdR concentration of approximately 1 micron is optimal. Autoradiographic exposure for 1 week or less is sufficient for TLI measurements on human tissues. With 3 to 4 atmospheres oxygen tension, incorporation of 3H-TdR is sufficient for TLI measurement throughout slices of tissue cut 1 mm thick or less. Mincing of tissue is not necessary, and the anatomic continuity seen in ordinary histological preparations is preserved. A gradient of labeling intensity is present from the surface to the interior of the tissue, but sufficient intensity of labeling for detection of DNA synthesis can be achieved in the interior of the section. The gradient can be reduced only slightly by prior incubation in 3H-TdR with hyperbaric oxygen at 0 C. The method permits TLI measurements on the same specimens, including needle biopsies, that are used for pathologic diagnosis.

摘要

实体组织胸苷标记指数(TLI)的体外测量需要高压氧合,并且通过5-氟-2'-脱氧尿苷(FUdR)对胸苷酸合成酶的阻断作用来增强,以利于氚标记胸苷(3H-TdR)的摄取。通过向带有橡胶塞的试管中注入氧气,可在一个简单的系统中实现高压氧合。孵育在含有汉克斯平衡盐溶液的摇床水浴中于37℃进行2小时;约1微摩尔的FUdR浓度最为适宜。对于人体组织的TLI测量,1周或更短时间的放射自显影曝光就足够了。在3至4个大气压的氧张力下,3H-TdR的掺入量足以对厚度为1毫米或更薄的组织切片进行TLI测量。无需将组织切碎,并且能保持普通组织学切片中可见的解剖学连续性。从组织表面到内部存在标记强度梯度,但在切片内部也能实现足以检测DNA合成的标记强度。在0℃下用3H-TdR和高压氧进行预孵育,只能略微降低这种梯度。该方法允许对用于病理诊断的相同标本(包括针吸活检标本)进行TLI测量。

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