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定制荧光核苷酸合成作为核酸标记的替代方法。

Custom fluorescent-nucleotide synthesis as an alternative method for nucleic acid labeling.

作者信息

Henegariu O, Bray-Ward P, Ward D C

机构信息

Department of Genetics, Yale University School of Medicine, 333 Cedar Street, New Haven, CT 06510, USA.

出版信息

Nat Biotechnol. 2000 Mar;18(3):345-8. doi: 10.1038/73815.

Abstract

The variety of potentially useful dyes or haptenes available for fluorescent nucleic acid hybridization assays is far greater than what can be obtained from commercial sources. Since this diversity could be useful in many laboratory applications, we have developed a simple and inexpensive procedure for preparing nonpurified labeled nucleotides, for use in common nucleic acid labeling reactions, such as PCR and nick translation. The modified nucleotides were synthesized by coupling allylamine-dUTP to the succinimidyl-ester derivatives of the fluorescent dyes or haptenes such as biotin or digoxigenin, which require fluorescently labeled proteins for detection. This method allows custom preparation of most common fluorescent nucleotides and rapid testing of new ones, while reducing the cost of procedures such as multiplex fluorescent in situ hybridization (M-FISH) by 100-200 fold.

摘要

可用于荧光核酸杂交检测的潜在有用染料或半抗原种类,远远超过从商业渠道所能获得的种类。鉴于这种多样性在许多实验室应用中可能有用,我们开发了一种简单且成本低廉的方法来制备未纯化的标记核苷酸,用于常见的核酸标记反应,如聚合酶链反应(PCR)和切口平移。通过将烯丙胺 - dUTP与荧光染料或半抗原(如生物素或地高辛)的琥珀酰亚胺酯衍生物偶联来合成修饰的核苷酸,这些半抗原检测时需要荧光标记蛋白。该方法允许定制制备大多数常见的荧光核苷酸,并能快速测试新的荧光核苷酸,同时将多重荧光原位杂交(M - FISH)等检测程序的成本降低100 - 200倍。

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