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大鼠甲状腺中降钙素信使核糖核酸的特性与定位

Characterization and localization of calcitonin messenger ribonucleic acid in rat thyroid.

作者信息

Jacobs J W, Simpson E, Penschow J, Hudson P, Coghlan J, Niall H

出版信息

Endocrinology. 1983 Nov;113(5):1616-22. doi: 10.1210/endo-113-5-1616.

Abstract

DNA/RNA hybridization assays have been used to examine calcitonin (CT) RNA production in normal rat thyroids. A cloned CT cDNA which codes for the entire rat CT precursor was radiolabeled to a high specific activity and used in hybridization assays to explore 1) the sizes and relative quantities of CT RNA extractable from thyroids obtained from rats of differing ages; 2) the effect of calcium on the in vitro production of CT RNA in rat thyroid tissue slices; and 3) the localization, by hybridization histochemistry, of C cells in rat thyroid that contain CT RNA. The relative concentrations of CT RNA, per microgram of total thyroid RNA, increased remarkably with age, with 14-month-old rats having approximately 14-fold elevated concentrations of thyroidal CT RNA compared to 19-day-old rat fetuses. Of interest was the finding that a second larger species of CT RNA is only evident in thyroids obtained from 14-month-old animals. The effect of calcium on the in vitro production of CT RNA in rat thyroid tissues was studied over 3- and 6-h periods. Although previous investigations have shown that calcium causes an immediate and linear increase in CT secretion from the thyroid gland, no net increase vs. controls in the amount of CT RNA extractable from calcium-stimulated thyroid slices was observed. Finally, hybridization histochemistry, a technique that identifies in fixed tissue sections those areas that contain a specific mRNA population, was used to localize C cells in the thyroid containing CT RNA. Specific areas of rat thyroid hybridized with the CT cDNA probe and autoradiography revealed these areas to be parafollicular cells located only in the central portion of the thyroid lobes, mRNA quantities detected by hybridization histochemistry showed little variation over the central area of the thyroid, indicating the C cells in this region of the thyroid are accumulating CT RNA at approximately the same rate.

摘要

DNA/RNA杂交试验已被用于检测正常大鼠甲状腺中降钙素(CT)RNA的产生。一个编码完整大鼠CT前体的克隆CT cDNA被放射性标记至高比活度,并用于杂交试验,以探究:1)从不同年龄大鼠的甲状腺中提取的CT RNA的大小和相对量;2)钙对大鼠甲状腺组织切片中CT RNA体外产生的影响;3)通过杂交组织化学定位大鼠甲状腺中含有CT RNA的C细胞。每微克总甲状腺RNA中CT RNA的相对浓度随年龄显著增加,14个月大的大鼠甲状腺CT RNA浓度比19天大的大鼠胎儿高约14倍。有趣的是,发现另一种更大的CT RNA仅在14个月大动物的甲状腺中明显。在3小时和6小时的时间段内研究了钙对大鼠甲状腺组织中CT RNA体外产生的影响。尽管先前的研究表明钙会导致甲状腺CT分泌立即呈线性增加,但未观察到与对照组相比,从钙刺激的甲状腺切片中可提取的CT RNA量有净增加。最后,杂交组织化学是一种在固定组织切片中识别含有特定mRNA群体区域的技术,用于定位甲状腺中含有CT RNA的C细胞。大鼠甲状腺的特定区域与CT cDNA探针杂交,放射自显影显示这些区域是仅位于甲状腺叶中央部分的滤泡旁细胞,通过杂交组织化学检测到的mRNA量在甲状腺中央区域变化很小,表明甲状腺该区域的C细胞以大致相同的速率积累CT RNA。

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