CRISPR-Cas immunity: analysis of adaptation and interference reactions in prokaryotes

Mobile genetic elements (MGEs, e.g. transposons, plasmids and phage) are an important driver of genetic diversity in microorganisms, and have diverse effects on microbe populations. Adaptation of Bacteria and Archaea to overcome negative effects of phage infection is sometimes referred to as an “arm...

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Main Author: Cass, S.D.B.
Format: Thesis (University of Nottingham only)
Language:English
Published: 2016
Subjects:
Online Access:https://eprints.nottingham.ac.uk/35784/
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author Cass, S.D.B.
author_facet Cass, S.D.B.
author_sort Cass, S.D.B.
building Nottingham Research Data Repository
collection Online Access
description Mobile genetic elements (MGEs, e.g. transposons, plasmids and phage) are an important driver of genetic diversity in microorganisms, and have diverse effects on microbe populations. Adaptation of Bacteria and Archaea to overcome negative effects of phage infection is sometimes referred to as an “arms race” that provokes the development of systems to protect against phage attack. One such defence is CRISPR-Cas, the topic of this research thesis. CRISPR (Clustered Regular Interspersed Short Palindromic Repeat) loci and Cas (CRISPR-associated) proteins are the molecular basis of this resistance mechanism. CRISPR-Cas can protect against phage and other foreign MGEs by incorporating a fragment of novel DNA into CRISPR (spacer acquisition) and using this as a template to generate a small RNA molecule, CRISPR RNA (crRNA), which targets the degradation of complementary sequences (interference). Effective interference requires formation of R-loop nucleic acid structure of crRNA base-pairing to homologous DNA, at positions flanked by PAM (Protospacer Adjacent Motif) sequence within the invader. This thesis investigates actions of CRISPR-Cas interference proteins, with focus on archaeal species Methanothermobacter thermautotrophicus (Mth) and Haloferax volcanii (Hvo). Mth and Hvo catalyse interference by utilizing a Cascade (CRISPR-associated Complex for Antiviral DEfence) protein-crRNA complex. Cas8, the large subunit protein in Cascade, was investigated to explain it’s essential role in interference. It is a PAM sensing protein that stabilizes R-loop formation to bring about interference. In addition, this analysis identified a surprising RNase activity of Cas8 that remains of unknown function. The thesis also details recent work on adaptation by Cas1 and Cas2 in Escherichia coli. Cas1 nuclease and transesterification activities upon replication fork intermediates are presented alongside a new model for spacer acquisition.
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format Thesis (University of Nottingham only)
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institution University of Nottingham Malaysia Campus
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language English
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spelling nottingham-357842025-02-28T11:50:24Z https://eprints.nottingham.ac.uk/35784/ CRISPR-Cas immunity: analysis of adaptation and interference reactions in prokaryotes Cass, S.D.B. Mobile genetic elements (MGEs, e.g. transposons, plasmids and phage) are an important driver of genetic diversity in microorganisms, and have diverse effects on microbe populations. Adaptation of Bacteria and Archaea to overcome negative effects of phage infection is sometimes referred to as an “arms race” that provokes the development of systems to protect against phage attack. One such defence is CRISPR-Cas, the topic of this research thesis. CRISPR (Clustered Regular Interspersed Short Palindromic Repeat) loci and Cas (CRISPR-associated) proteins are the molecular basis of this resistance mechanism. CRISPR-Cas can protect against phage and other foreign MGEs by incorporating a fragment of novel DNA into CRISPR (spacer acquisition) and using this as a template to generate a small RNA molecule, CRISPR RNA (crRNA), which targets the degradation of complementary sequences (interference). Effective interference requires formation of R-loop nucleic acid structure of crRNA base-pairing to homologous DNA, at positions flanked by PAM (Protospacer Adjacent Motif) sequence within the invader. This thesis investigates actions of CRISPR-Cas interference proteins, with focus on archaeal species Methanothermobacter thermautotrophicus (Mth) and Haloferax volcanii (Hvo). Mth and Hvo catalyse interference by utilizing a Cascade (CRISPR-associated Complex for Antiviral DEfence) protein-crRNA complex. Cas8, the large subunit protein in Cascade, was investigated to explain it’s essential role in interference. It is a PAM sensing protein that stabilizes R-loop formation to bring about interference. In addition, this analysis identified a surprising RNase activity of Cas8 that remains of unknown function. The thesis also details recent work on adaptation by Cas1 and Cas2 in Escherichia coli. Cas1 nuclease and transesterification activities upon replication fork intermediates are presented alongside a new model for spacer acquisition. 2016-12-15 Thesis (University of Nottingham only) NonPeerReviewed application/pdf en arr https://eprints.nottingham.ac.uk/35784/1/Cass%20Thesis%20V3.pdf Cass, S.D.B. (2016) CRISPR-Cas immunity: analysis of adaptation and interference reactions in prokaryotes. PhD thesis, University of Nottingham. CRISPR Cas8 Cas1 Cas2 Biochemistry Proteins DNA Archaea Bacteria Molecular biology
spellingShingle CRISPR
Cas8
Cas1
Cas2
Biochemistry
Proteins
DNA
Archaea
Bacteria
Molecular biology
Cass, S.D.B.
CRISPR-Cas immunity: analysis of adaptation and interference reactions in prokaryotes
title CRISPR-Cas immunity: analysis of adaptation and interference reactions in prokaryotes
title_full CRISPR-Cas immunity: analysis of adaptation and interference reactions in prokaryotes
title_fullStr CRISPR-Cas immunity: analysis of adaptation and interference reactions in prokaryotes
title_full_unstemmed CRISPR-Cas immunity: analysis of adaptation and interference reactions in prokaryotes
title_short CRISPR-Cas immunity: analysis of adaptation and interference reactions in prokaryotes
title_sort crispr-cas immunity: analysis of adaptation and interference reactions in prokaryotes
topic CRISPR
Cas8
Cas1
Cas2
Biochemistry
Proteins
DNA
Archaea
Bacteria
Molecular biology
url https://eprints.nottingham.ac.uk/35784/