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Deoxyribonucleic Acid-Deoxyribonucleic Acid Hybridization Assay for Replication Origin Deoxyribonucleic Acid of Escherichia coli

机译:脱氧核糖核酸 - 脱氧核糖核酸杂交测定用于复制源性大肠杆菌的脱氧核糖核酸

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Deoxyribonucleic acid (DNA)-DNA hybridization on nitrocellulose filters can be used to assay for replication origin DNA from Escherichia coli if the DNA attached to the filters is enriched for the replication origin sequences. Such DNA can be readily isolated from very rapidly growing cells. When low amounts of this DNA were attached to filters, radioactively labeled DNA from the replication origin hybridized 1.7 times as well as radioactive replication terminus DNA. Under identical conditions, radioactively labeled DNA from exponentially growing cells hybridized only 1.3 times as well as radioactive replication terminus DNA. The replication origin, replication terminus, and randomly labeled DNA hybridized with similar efficiencies to filters containing DNA isolated from cells incubated in the absence of required amino acids. This DNA appeared to have all sequences present at equal frequencies. The hybridization assay was used to demonstrate that the DNA synthesized shortly after the addition of amino acids to cells previously deprived of required amino acids was primarily from the replication origin and then rapidly became similar to DNA synthesized by exponentially growing cells.
机译:硝酸核核酸(DNA)-DNA杂交硝酸纤维素过滤器可用于测定来自大肠杆菌的复制源DNA,如果附着到过滤器的DNA富集为复制来源序列。这种DNA可以容易地从非常快速生长的细胞中分离出来。当将该DNA的低量连接到过滤器时,从复制源杂交的放射性标记的DNA杂交1.7倍以及放射性复制末端DNA。在相同的条件下,来自指数生长细胞的放射性标记的DNA仅杂交只有1.3倍以及放射性复制末端DNA。复制起源,复制末端和随机标记的DNA与类似效率的杂交杂交,以在不存在所需氨基酸的情况下孵育的细胞中分离的DNA的过滤器。该DNA似乎具有在等频率时存在的所有序列。杂交测定用于证明在将氨基酸加入以前剥夺所需氨基酸的氨基酸后不久合成的DNA主要来自复制来源,然后快速变为与通过指数生长细胞合成的DNA。

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