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用于限制性片段序列分析的共价连接测序引物接头(splinkers)

Covalently linked sequencing primer linkers (splinkers) for sequence analysis of restriction fragments.

作者信息

Kalisch B W, Krawetz S A, Schoenwaelder K H, van de Sande J H

出版信息

Gene. 1986;44(2-3):263-70. doi: 10.1016/0378-1119(86)90190-3.

Abstract

A new method for direct sequence analysis of DNA restriction fragments uses synthetic covalently linked complementary oligodeoxynucleotides, as universal sequencing primer linkers (splinkers). These splinkers were designed to contain an inverted repeat sequence which forms a double-stranded hairpin structure with a known restriction site. The splinkers were characterized by their ability to be self-ligating (dimerized) and by their restriction digest product analysis of both the monomer and dimer. They can also be ligated to dephosphorylated DNA restriction fragments which contain the appropriate end. This was evidenced by mobility shifts of the splinker-ligated restriction fragments. The splinker-ligated restriction fragments, after denaturation, form a single-stranded DNA template containing an inverted repeat sequence (from splinker) at one terminus. The splinker is thus suitably oriented and serves as a primer for dideoxy nucleotide (nt) sequencing catalyzed by either Klenow fragment of Escherichia coli DNA polymerase I or avian myeloblastosis virus reverse transcriptase. As demonstrated for both pBR322 and phi X174, release of the primer extension strand by digestion at the splinker restriction site results in a ladder of labelled fragments which corresponds to a unique nt sequence.

摘要

一种用于DNA限制性片段直接序列分析的新方法,使用合成的共价连接的互补寡脱氧核苷酸作为通用测序引物连接体(splinkers)。这些splinkers被设计成含有一个反向重复序列,该序列与一个已知的限制性位点形成双链发夹结构。splinkers的特征在于它们的自我连接(二聚化)能力以及对单体和二聚体的限制性消化产物分析。它们还可以连接到含有适当末端的去磷酸化DNA限制性片段上。这通过splinker连接的限制性片段的迁移率变化得到证明。变性后,splinker连接的限制性片段形成一个单链DNA模板,其一端含有一个反向重复序列(来自splinker)。因此,splinker的方向合适,并作为由大肠杆菌DNA聚合酶I的Klenow片段或禽成髓细胞瘤病毒逆转录酶催化的双脱氧核苷酸(nt)测序的引物。正如对pBR322和phi X174所证明的那样,通过在splinker限制性位点进行消化来释放引物延伸链,会产生一系列标记片段,这些片段对应于一个独特的nt序列。

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