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用于原位杂交的3'和5'生物素标记寡核苷酸的比较

Comparison of 3' and 5' biotin labelled oligonucleotides for in situ hybridisation.

作者信息

Bardin P G, Pickett M A, Robinson S B, Sanderson G, Holgate S T, Johnston S L

机构信息

Immunopharmacology Group, University Medicine, Southampton General Hospital, UK.

出版信息

Histochemistry. 1993 Nov;100(5):387-92. doi: 10.1007/BF00268937.

Abstract

Oligonucleotide probes enzymatically labelled at the 3'-end with biotin have been used successfully to detect target RNA and DNA in combination with in situ hybridisation. Addition of multiple biotin residues to the 3'-end increases the hybridisation signals, but it is not known whether the same principle is applicable to the 5'-end. We have labelled a 35-base oligonucleotide during synthesis with 1, 5 and 12 biotin molecules at the 5'-end and compared it to conventional 3'-labelling. In additional experiments the probes were labelled at both ends. Probes were applied to histological sections obtained from paraffin-embedded cell-clot-complexes that contain uninfected and Rhinoviral-infected cells, using a standard in situ hybridisation protocol with appropriate controls. Hybridisation signals were compared for intensity of cytoplasmic signal and sensitivity as number of positive cells. Both parameters increased in parallel with higher numbers of biotin residues attached to the 5'-end and 12 biotin residues were almost as effective as 3'-enzymatic tailing. The sensitivity could be increased above that of either 3'- or 5'-labelling by the addition of residues at both ends of the probe. The 5'-attachment of biotin residues can extend the value of oligonucleotide probes employed for in situ hybridisation and yield increased sensitivity when combined with 3'-enzymatic labelling.

摘要

3'端用生物素酶促标记的寡核苷酸探针已成功用于结合原位杂交检测靶RNA和DNA。在3'端添加多个生物素残基可增加杂交信号,但尚不清楚相同原理是否适用于5'端。我们在合成过程中用1个、5个和12个生物素分子在5'端标记了一个35个碱基的寡核苷酸,并将其与传统的3'端标记进行了比较。在额外的实验中,探针在两端都进行了标记。使用标准原位杂交方案并设置适当对照,将探针应用于从石蜡包埋的细胞凝块复合物中获得的组织学切片,这些复合物包含未感染和鼻病毒感染的细胞。比较杂交信号的细胞质信号强度和作为阳性细胞数量的灵敏度。这两个参数都随着5'端连接的生物素残基数量增加而平行增加,并且12个生物素残基几乎与3'端酶促加尾一样有效。通过在探针两端添加残基,灵敏度可以提高到高于3'端或5'端标记的水平。在寡核苷酸探针5'端连接生物素残基可以扩展用于原位杂交的寡核苷酸探针的价值,并在与3'端酶促标记结合时提高灵敏度。

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