| 半随机单引物PCR扩增产物的特异性研究 |
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| 引用本文: | 杨树青,徐迅.半随机单引物PCR扩增产物的特异性研究[J].复旦学报(自然科学版),1994,33(2):121-126. |
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| 作者姓名: | 杨树青 徐迅 |
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| 作者单位: | 复旦大学遗传学研究所 |
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| 摘 要: | 以M13mp19为模板,寡核苷酸“1224”为引物,进行半随机单引物PCR扩增;分析其扩增产物的限制性内切酶酶切图谱,推定它们分别在M13mp19序列中的确切位置;证实引物“1224”的3端与模板M13mp19负链的互补结合,至少需有连续的4上个核苷酸,才能产生单引物PCR扩增的模板分子,进行有效的PCR扩增,并由此决定了扩增产物中各DNA片段的大小及其在模板DNA序列中的特定位置。
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| 关 键 词: | 扩增 聚合酶 遗传工程 单引物 PCR |
Study on the specificity of amplification products by single-primer PCR |
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| Yang Shuqing, Xu Xun, Zhang Hong, Mao YuminLao Ye, Wen Jun''''e, Wang Xianmin.Study on the specificity of amplification products by single-primer PCR[J].Journal of Fudan University(Natural Science),1994,33(2):121-126. |
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| Authors: | Yang Shuqing Xu Xun Zhang Hong Mao YuminLao Ye Wen Jun'e Wang Xianmin |
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| Institution: | Institute of Genetics |
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| Abstract: | The template M,13mp19 was amplified by the semi-random single-primer PCR with the oligonucleotide primer "1224", The DNA fragments in the amplification products were purified and used as the templates. The latter was then amplified by the same single-primer PCR under the normal condition. The exact regions where these products were located and the starting sites of the specific PCR amplification were determined. It was shown that more than 4 nucleotides at the 3,termination of the primer"1224" integrating complementarily with the template DNA were needed for the production of the template molecules of single-primer PCR and the effective PCR amplification. Moreover, the sites of integration determined the lengths of DNA fragments in the amplification products and their specific locations in the template DNA. |
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| Keywords: | primer amplification polymcrase restriction endonucleases polymerasc chain reaction single-primer PCR amplification |
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