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核苷酸序列上结合位点的信息内容。

Information content of binding sites on nucleotide sequences.

作者信息

Schneider T D, Stormo G D, Gold L, Ehrenfeucht A

出版信息

J Mol Biol. 1986 Apr 5;188(3):415-31. doi: 10.1016/0022-2836(86)90165-8.

Abstract

Repressors, polymerases, ribosomes and other macromolecules bind to specific nucleic acid sequences. They can find a binding site only if the sequence has a recognizable pattern. We define a measure of the information (R sequence) in the sequence patterns at binding sites. It allows one to investigate how information is distributed across the sites and to compare one site to another. One can also calculate the amount of information (R frequency) that would be required to locate the sites, given that they occur with some frequency in the genome. Several Escherichia coli binding sites were analyzed using these two independent empirical measurements. The two amounts of information are similar for most of the sites we analyzed. In contrast, bacteriophage T7 RNA polymerase binding sites contain about twice as much information as is necessary for recognition by the T7 polymerase, suggesting that a second protein may bind at T7 promoters. The extra information can be accounted for by a strong symmetry element found at the T7 promoters. This element may be an operator. If this model is correct, these promoters and operators do not share much information. The comparisons between R sequence and R frequency suggest that the information at binding sites is just sufficient for the sites to be distinguished from the rest of the genome.

摘要

阻遏蛋白、聚合酶、核糖体及其他大分子会与特定的核酸序列结合。只有当序列具有可识别的模式时,它们才能找到结合位点。我们定义了一种针对结合位点处序列模式中信息(R序列)的度量方法。它能让人研究信息在各个位点上是如何分布的,以及将一个位点与另一个位点进行比较。人们还可以计算出在已知这些位点在基因组中以一定频率出现的情况下,定位这些位点所需的信息量(R频率)。使用这两种独立的实证测量方法对多个大肠杆菌结合位点进行了分析。对于我们分析的大多数位点而言,这两种信息量是相似的。相比之下,噬菌体T7 RNA聚合酶结合位点所包含的信息大约是T7聚合酶识别所需信息量的两倍,这表明可能有第二种蛋白质会结合在T7启动子上。额外的信息可以由在T7启动子处发现的一个强对称元件来解释。这个元件可能是一个操纵基因。如果这个模型是正确的,那么这些启动子和操纵基因并没有共享太多信息。R序列和R频率之间的比较表明,结合位点处的信息刚好足以使这些位点与基因组的其他部分区分开来。

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