In vivo investigation of interactions between replisome components in Escherichia coli: An expanded model for the processivity switch
Background: Protein interactions within the replisome (a highly coordinated protein complex) are crucial to maintain temporal and spatial regulation for high fidelity DNA synthesis in Escherichia coli (E. coli). A key component of these interactions is the processivity switch, ensuring smooth transi...
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University of the Punjab
2020-02-01
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| Series: | Advancements in Life Sciences |
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| Online Access: | http://www.als-journal.com/723-20/ |
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doaj-424e47f59a624aedb406544950ba7e8e2020-11-25T01:10:36Zeng University of the PunjabAdvancements in Life Sciences2310-53802310-53802020-02-01726671In vivo investigation of interactions between replisome components in Escherichia coli: An expanded model for the processivity switchAtif A. Patoli0School of Biology, Queens Medical Centre, University of Nottingham, Nottingham – UKBackground: Protein interactions within the replisome (a highly coordinated protein complex) are crucial to maintain temporal and spatial regulation for high fidelity DNA synthesis in Escherichia coli (E. coli). A key component of these interactions is the processivity switch, ensuring smooth transition of the replicative DNA polymerase III (Pol III) between Okazaki fragments on the lagging strand. Multiple interaction studies between replisome components have been performed to indicate the essential roles of Pol III (DnaE), β-clamp, DnaB helicase, DNA and the t (DnaX) subunit for this switch. Methods: Known interacting regions of both DnaE and various truncated versions of t were chosen for co-expression in E. coli. Differences in the growth pattern of cells co-expressing various truncated versions of DnaX and DnaE, on liquid and solid media were subsequently analyzed. Based on in vivo analyses to explore the interactions between these components, an expanded model for the processivity switch is presented here. Results: The analyses suggest that residues 481-643 of t are sufficient to establish a functional interaction with the DnaB helicase and DnaE during replication, while residues 461-480 of t interact with the C-terminal tail of DnaE to disengage Pol III from the β-clamp during processivity switching. We also propose that residues 430-460 of t are involved in sensing the DNA structure required for the processivity switch. Conclusion: These observations expand the current understanding of processivity switching and help dissect the regions of t utilized for binding to different replisome components such as DnaB helicase, polymerase and DNA.http://www.als-journal.com/723-20/processivity switchclamp loaderdnaednaxdnab helicase |
| collection |
DOAJ |
| language |
English |
| format |
Article |
| sources |
DOAJ |
| author |
Atif A. Patoli |
| spellingShingle |
Atif A. Patoli In vivo investigation of interactions between replisome components in Escherichia coli: An expanded model for the processivity switch Advancements in Life Sciences processivity switch clamp loader dnae dnax dnab helicase |
| author_facet |
Atif A. Patoli |
| author_sort |
Atif A. Patoli |
| title |
In vivo investigation of interactions between replisome components in Escherichia coli: An expanded model for the processivity switch |
| title_short |
In vivo investigation of interactions between replisome components in Escherichia coli: An expanded model for the processivity switch |
| title_full |
In vivo investigation of interactions between replisome components in Escherichia coli: An expanded model for the processivity switch |
| title_fullStr |
In vivo investigation of interactions between replisome components in Escherichia coli: An expanded model for the processivity switch |
| title_full_unstemmed |
In vivo investigation of interactions between replisome components in Escherichia coli: An expanded model for the processivity switch |
| title_sort |
in vivo investigation of interactions between replisome components in escherichia coli: an expanded model for the processivity switch |
| publisher |
University of the Punjab |
| series |
Advancements in Life Sciences |
| issn |
2310-5380 2310-5380 |
| publishDate |
2020-02-01 |
| description |
Background: Protein interactions within the replisome (a highly coordinated protein complex) are crucial to maintain temporal and spatial regulation for high fidelity DNA synthesis in Escherichia coli (E. coli). A key component of these interactions is the processivity switch, ensuring smooth transition of the replicative DNA polymerase III (Pol III) between Okazaki fragments on the lagging strand. Multiple interaction studies between replisome components have been performed to indicate the essential roles of Pol III (DnaE), β-clamp, DnaB helicase, DNA and the t (DnaX) subunit for this switch.
Methods: Known interacting regions of both DnaE and various truncated versions of t were chosen for co-expression in E. coli. Differences in the growth pattern of cells co-expressing various truncated versions of DnaX and DnaE, on liquid and solid media were subsequently analyzed. Based on in vivo analyses to explore the interactions between these components, an expanded model for the processivity switch is presented here.
Results: The analyses suggest that residues 481-643 of t are sufficient to establish a functional interaction with the DnaB helicase and DnaE during replication, while residues 461-480 of t interact with the C-terminal tail of DnaE to disengage Pol III from the β-clamp during processivity switching. We also propose that residues 430-460 of t are involved in sensing the DNA structure required for the processivity switch.
Conclusion: These observations expand the current understanding of processivity switching and help dissect the regions of t utilized for binding to different replisome components such as DnaB helicase, polymerase and DNA. |
| topic |
processivity switch clamp loader dnae dnax dnab helicase |
| url |
http://www.als-journal.com/723-20/ |
| work_keys_str_mv |
AT atifapatoli invivoinvestigationofinteractionsbetweenreplisomecomponentsinescherichiacolianexpandedmodelfortheprocessivityswitch |
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