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Novel chemical method for the preparation of nucleic acids for nonisotopic hybridization.

机译:制备用于非同位素杂交的核酸的新型化学方法。

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摘要

A novel chemical method was used to prepare biotin-labeled nucleic acids for nonisotopic hybridization. The method involves the transamination of unpaired cytosine residues in polynucleotides with sodium bisulfite and ethylenediamine. Primary amino groups on the cytosine derivatives are then reacted with biotinyl-e-aminocaproic acid N-hydroxysuccinimide ester. Biotinylated probes hybridized with 1 to 2 pg of nitrocellulose filter-bound DNA and were visualized with a colorimetric detection technique. This method is simpler and less expensive than other methods for the preparation of nonisotopic probes. In addition, it is more versatile since the chemically modified bases can potentially react with other "indicator" molecules or proteins such as an enzyme. The specificity for unpaired cytosine residues is another advantage which could allow for the selective labeling of a specific region of a double-stranded nucleic acid. This improved labeling method should lead to the wider application of hybridization techniques in diagnostic microbiology and basic research in infectious diseases.
机译:一种新颖的化学方法被用来制备生物素标记的核酸用于非同位素杂交。该方法涉及用亚硫酸氢钠和乙二胺对多核苷酸中未配对的胞嘧啶残基进行氨基转移。然后,将胞嘧啶衍生物上的伯氨基与生物素-e-氨基己酸N-羟基琥珀酰亚胺酯反应。生物素化探针与1至2 pg硝酸纤维素滤膜结合的DNA杂交,并通过比色检测技术进行可视化。该方法比其他制备非同位素探针的方法更简单,更便宜。另外,它更通用,因为化学修饰的碱基可以潜在地与其他“指示剂”分子或蛋白质(例如酶)反应。未配对的胞嘧啶残基的特异性是另一个优点,其可以允许选择性标记双链核酸的特定区域。这种改进的标记方法应导致杂交技术在诊断微生物学和传染病基础研究中的广泛应用。

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