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一种基于汞化核酸探针和巯基半抗原配体的新型杂交细胞化学方法。II. 配体结构变化对汞化探针原位检测的影响。

A new hybridocytochemical method based on mercurated nucleic acid probes and sulfhydryl-hapten ligands. II. Effects of variations in ligand structure on the in situ detection of mercurated probes.

作者信息

Hopman A H, Wiegant J, van Duijn P

出版信息

Histochemistry. 1986;84(2):179-85. doi: 10.1007/BF00499830.

Abstract

In the preceding paper, a method to detect specific DNA sequences with mercurated nucleic acid probes and sulfhydryl-hapten ligands has been described. Due to the instability of the bond between mercury and a negatively charged sulfhydryl-hapten ligand (trinitrophenyl-glutathione), the in situ formed hybrid could not be detected. On basis of model system experiments it was suggested that this mercury-sulfhydryl bond could be stabilized by an extra polar interaction between ligand and nucleic acid. This was achieved by reversing the net charge of the ligand. Such ligands were synthesized by reacting aliphatic diamines to the carboxyl groups of Tnp-glutathione using a water soluble carbodiimide. Gel chromatographic analysis of mercurated polynucleotide-ligand complexes showed that the stability of the mercury-sulfhydryl bond is increased by the reversal of the net charge of the ligand. In situ hybridized mercurated mouse satellite DNA to mouse liver nuclei and mercurated kinetoplast cRNA hybridized to Crithidia fasciculata were immunocytochemically detected after the introduction of these positively charged ligands. The described method is applicable for RNA and DNA probes. It has a sensitivity comparable to other non-autoradiographic methods, is relatively simple to perform and can be carried out with ordinary laboratory chemicals.

摘要

在前一篇论文中,已经描述了一种使用汞化核酸探针和巯基半抗原配体检测特定DNA序列的方法。由于汞与带负电荷的巯基半抗原配体(三硝基苯基-谷胱甘肽)之间的键不稳定,原位形成的杂交体无法被检测到。基于模型系统实验,有人提出这种汞-巯基键可以通过配体与核酸之间额外的极性相互作用来稳定。这是通过反转配体的净电荷来实现的。此类配体是通过使用水溶性碳二亚胺使脂肪族二胺与Tnp-谷胱甘肽的羧基反应合成的。对汞化多核苷酸-配体复合物的凝胶色谱分析表明,配体净电荷的反转增加了汞-巯基键的稳定性。在引入这些带正电荷的配体后,通过免疫细胞化学方法检测到了原位杂交的汞化小鼠卫星DNA与小鼠肝细胞核以及汞化动质体cRNA与克氏锥虫的杂交情况。所描述的方法适用于RNA和DNA探针。它具有与其他非放射自显影方法相当的灵敏度,操作相对简单,并且可以使用普通的实验室化学试剂进行。

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