The Escherichia coli DnaK chaperone stimulates the α-complementation of β-galactosidase.

J Basic Microbiol

Department of Computational Biology and Medical Sciences, Graduate School of Frontier Sciences, The University of Tokyo, Kashiwa, Japan.

Published: June 2022

AI Article Synopsis

  • pUC18 and pUC19 are common plasmid vectors used for DNA cloning, with differences in their α-complementation efficiency of β-galactosidase.
  • The α-complementation for pUC18 (via LacZα18) is weak and requires the DnaK chaperone system for enhancement, while pUC19 (via LacZα19) operates efficiently without DnaK.
  • These findings suggest that DnaK enhances, but isn't essential for α-complementation, and could facilitate new methods for screening DnaK inhibitors and understanding protein quality control.

Article Abstract

pUC18 and pUC19 are well-known high copy-number plasmid vectors routinely used for DNA cloning purposes. We show here that, in Escherichia coli transformed by native pUC18, the α-complementation of β-galactosidase (i.e., mediated by the peptide LacZα18) is intrinsically weak and slow, but is greatly stimulated by the DnaK/DnaJ/GrpE chaperone system. In contrast, the α-complementation mediated by the peptide LacZα19 (in E. coli transformed by the native pUC19) is much more efficient and therefore does not require the assistance of the DnaK chaperone machinery. The marked difference between these two LacZα peptides is reproduced in a cell-free protein expression system coupled with α-complementation. We conclude that: (i) α-complementation of β-galactosidase is DnaK-mediated depending upon the LacZα peptide donor; (ii) DnaK, sensu stricto, is not necessary for α-complementation, but can enhance it to a great extent; (iii) this observation could be used to establish an easy and inexpensive method for screening small molecules libraries in search of DnaK inhibitors and also for deciphering the DnaK-mediated protein quality control mechanism.

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Source
http://dx.doi.org/10.1002/jobm.202100487DOI Listing

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