Suppr超能文献

可在单一特定位点产生切口的质粒克隆载体。

Plasmid cloning vectors that can be nicked at a unique site.

作者信息

Bishop J O, Davies J A

出版信息

Mol Gen Genet. 1980;179(3):573-80. doi: 10.1007/BF00271747.

Abstract

We describe ColEl-type plasmids, with relaxed DNA replication, based on pMB9, and carrying the CmR determinant of R1, in addition to the TcR determinant of pMB9. One of the plasmids, pPH207, has unique sites for EcoRI, HindIII, BamI, SalI and HpaI. Insertion of foreign DNA into all but the last of these inactivates either the CmR or the TcR determinant. The original CmR TcR plasmid (pCM2) contains a copy of IS1 which produces deletions to left and to right. Most of these inactivate either the CmR or the TcR determinant. An internal 280 bp deletion of IS1 DNA in pPH207 greatly reduces the frequency at which deletions are observed. The main feature of these plasmids is a site that is cleaved by some preparations of EcoRI in only one strand of the DNA duplex (the EcoRIn site). This site facilitates strand separation of sequences inserted at the HindIII, BamI and SalI sites of the TcR gene, and also of any inserted at the true EcoRI site by a method that destroys that site. Since the orientation of the EcoRIn site is known, the orientation of sequences inserted at the neighbouring sites can be easily determined. Plasmid pPH207 is not mobilised by a Hfr, but its mobilisation is promoted by ColEl. It is therefore Mob- bom+. Experiments with minicells show that it directs the copious synthesis of chloramphenicol transacetylase.

摘要

我们描述了基于pMB9的具有松弛型DNA复制的ColEl型质粒,它除了携带pMB9的TcR决定簇外,还携带R1的CmR决定簇。其中一个质粒pPH207具有EcoRI、HindIII、BamI、SalI和HpaI的独特位点。将外源DNA插入除最后一个位点之外的所有这些位点中,会使CmR或TcR决定簇失活。原始的CmR TcR质粒(pCM2)包含一个IS1拷贝,该拷贝会产生向左和向右的缺失。其中大多数会使CmR或TcR决定簇失活。pPH207中IS1 DNA的280 bp内部缺失大大降低了观察到缺失的频率。这些质粒的主要特征是一个位点,某些EcoRI制剂仅在DNA双链的一条链上切割该位点(EcoRIn位点)。该位点有助于在TcR基因的HindIII、BamI和SalI位点插入的序列以及通过破坏该位点的方法在真正的EcoRI位点插入的任何序列的链分离。由于EcoRIn位点的方向已知,因此可以轻松确定在相邻位点插入的序列的方向。质粒pPH207不能被Hfr动员,但它的动员受到ColEl的促进。因此它是Mob- bom+。用微小细胞进行的实验表明,它指导氯霉素转乙酰酶的大量合成。

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