2018
DOI: 10.1371/journal.pone.0198564
|View full text |Cite
|
Sign up to set email alerts
|

Evidence for a second regulatory binding site on PspF that is occupied by the C-terminal domain of PspA

Abstract: PspA is a key component of the bacterial Psp membrane-stress response system. The biochemical and functional characterization of PspA is impeded by its oligomerization and aggregation properties. It was recently possible to solve the coiled coil structure of a completely soluble PspA fragment, PspA(1–144), that associates with the σ54 enhancer binding protein PspF at its W56-loop and thereby down-regulates the Psp response. We now found that the C-terminal part of PspA, PspA(145–222), also interacts with PspF … Show more

Help me understand this report

Search citation statements

Order By: Relevance

Paper Sections

Select...
1

Citation Types

0
1
0

Year Published

2018
2018
2022
2022

Publication Types

Select...
4

Relationship

1
3

Authors

Journals

citations
Cited by 4 publications
(1 citation statement)
references
References 27 publications
(92 reference statements)
0
1
0
Order By: Relevance
“…Site specific mutagenesis of pHIS1522- tcdB D286/288N ( Wohlan et al, 2014 ) was used to introduce a silent mutation in tcdB at postion A473 with the primer pair tcdB -sil-NdeI-F and tcdB -sil-NdeI-R, which eliminated an intrinsic NdeI-site, resulting in the vector pHIS1522- tcdB D286/288N silent NdeI. To analyze protein–protein interactions by the B2H screen, tcdE -M1, tcdL , and tcdB were amplified with the primer pairs 2H- tcdE -BamHI-F/2H- tcdE -KpnI-R, 2H- tcdB -BamHI-F/2H- tcdB -KpnI-R, and 2H- tcdL -BamHI-F/2H- tcdL -KpnI-R, and cloned into the corresponding sites of pU-strep- pspA (25–144)-T18, pUT18C- pspA (25–144)-strep, pK-strep- pspA (25–144)-T25, and pKT25- pspA (25–144)-strep ( Heidrich and Brüser, 2018 ). Single amino acid exchanges in TcdE for I151V were done as described above.…”
Section: Methodsmentioning
confidence: 99%
“…Site specific mutagenesis of pHIS1522- tcdB D286/288N ( Wohlan et al, 2014 ) was used to introduce a silent mutation in tcdB at postion A473 with the primer pair tcdB -sil-NdeI-F and tcdB -sil-NdeI-R, which eliminated an intrinsic NdeI-site, resulting in the vector pHIS1522- tcdB D286/288N silent NdeI. To analyze protein–protein interactions by the B2H screen, tcdE -M1, tcdL , and tcdB were amplified with the primer pairs 2H- tcdE -BamHI-F/2H- tcdE -KpnI-R, 2H- tcdB -BamHI-F/2H- tcdB -KpnI-R, and 2H- tcdL -BamHI-F/2H- tcdL -KpnI-R, and cloned into the corresponding sites of pU-strep- pspA (25–144)-T18, pUT18C- pspA (25–144)-strep, pK-strep- pspA (25–144)-T25, and pKT25- pspA (25–144)-strep ( Heidrich and Brüser, 2018 ). Single amino acid exchanges in TcdE for I151V were done as described above.…”
Section: Methodsmentioning
confidence: 99%