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Physical parameters affecting the rate and completion of RNA driven hybridization of DNA: new measurements relevant to quantitation based on kinetics.

机译:影响RNA驱动DNA杂交的速率和完成程度的物理参数:与基于动力学的定量相关的新测量值。

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摘要

Differences in the RNA-driven hybridization kinetics of genomic DNA and cDNA probes led us to examine physical parameters affecting these reactions. Cloned cDNA complementary to serum albumin (SA) mRNA hybridized in accordance with single component kinetics, whereas cloned SA genomic DNA hybridized more slowly and with multiple component kinetics. This difference is largely attributable to the relatively short and variable lengths of the mRNA complementary regions in the cloned genomic DNA. The rate of mRNA driven hybridization is affected to about half the extent observed for DNA renaturation as Na+ is increased or decreased from 0.18M. In the annealing of nucleic acids of high sequence complexity, after approximately 70% of reaction has been reached, the rate of the reaction is slowed and completion is not reached under "static" conditions. In practical terms, this is not the case for systems of low sequence complexity. This problem can be largely overcome by continuous or frequent mixing of the reactants, so that complex cDNA probes are hybridized essentially to completion, and kinetics can therefore be more readily compared to simple complexity standards.
机译:RNA驱动的基因组DNA和cDNA探针杂交动力学的差异使我们研究了影响这些反应的物理参数。克隆的与血清白蛋白(SA)mRNA互补的cDNA按照单组分动力学进行杂交,而克隆的SA基因组DNA杂交较慢且具有多组分动力学。该差异主要归因于克隆的基因组DNA中mRNA互补区域的相对较短和可变长度。当Na +从0.18M增加或减少时,mRNA驱动的杂交速率受到的影响约为DNA复性的一半。在高序列复杂性核酸的退火中,在达到大约70%的反应后,反应速度变慢并且在“静态”条件下未达到完成。实际上,对于低序列复杂度的系统不是这种情况。通过连续或频繁地混合反应物可以大大克服该问题,从而使复杂的cDNA探针基本上杂交至完全,因此与简单的复杂性标准物相比,动力学更容易。

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