Nielsen D A, Novoradovsky A, Goldman D
Section of Molecular Genetics, NIAAA, NIH, Bethesda, MD 20892-0001, USA.
Nucleic Acids Res. 1995 Jun 25;23(12):2287-91. doi: 10.1093/nar/23.12.2287.
To predict alterations in single-strand DNA mobility in non-denaturing electrophoretic gels, Zuker's RNA folding program was modified. Energy files utilized by the LRNA RNA folding algorithm were modified to emulate folding of single-strand DNA. Energy files were modified to disallow G-T base pairing. Stacking energies were corrected for DNA thermodynamics. Constraints on loop nucleotide sequences were removed. The LRNA RNA folding algorithm using the DNA fold energy files was applied to predict folding of PCR generated single-strand DNA molecules from polymorphic human ALDH2 and TPH alleles. The DNA-Fold version 1.0 program was used to design primers to create and abolish SSCP mobility shifts. Primers were made that add a 5' tag sequence or alter complementarity to an internal sequence. Differences in DNA secondary structure were assessed by SSCP analysis and compared to single-strand DNA secondary structure predictions. Results demonstrate that alterations in single-strand DNA conformation may be predicted using DNA-Fold 1.0.
为预测非变性电泳凝胶中单链DNA迁移率的变化,对祖克的RNA折叠程序进行了修改。对LRNA RNA折叠算法所使用的能量文件进行修改,以模拟单链DNA的折叠。修改能量文件以禁止G-T碱基配对。对堆积能量进行校正以符合DNA热力学。去除对环核苷酸序列的限制。使用DNA折叠能量文件的LRNA RNA折叠算法被应用于预测来自多态性人类ALDH2和TPH等位基因的PCR产生的单链DNA分子的折叠。使用DNA-Fold 1.0程序设计引物,以产生和消除SSCP迁移率变化。设计的引物添加了5'标签序列或改变了与内部序列的互补性。通过SSCP分析评估DNA二级结构的差异,并与单链DNA二级结构预测结果进行比较。结果表明,使用DNA-Fold 1.0可以预测单链DNA构象的变化。
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