Mini-Tn
 7
 Insertion in an Artificial
 att
 Tn
 7
 Site Enables Depletion of the Essential Master Regulator CtrA in the Phytopathogen Agrobacterium tumefaciens

Figueroa-Cuilan, Wanda M.; Daniel, Jeremy J.; Howell, Matthew; Sulaiman, Aliyah; Brown, Pamela

doi:10.1128/aem.01392-16

Cited by 45 publications

(48 citation statements)

References 51 publications

(65 reference statements)

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“…All scale bars are set to 2 µm. promoter at a neutral site in the chromosome (Figueroa-Cuilan et al, 2016;Howell and Brown, 2016). Using western blot analysis, we have confirmed the depletion of FtsZ AT in the absence of IPTG (Supplemental Fig.…”

Section: Resultssupporting

confidence: 62%

“…To characterize the function of each FtsZ homolog, we constructed deletions of ftsZ 1 and ftsZ 3 and a depletion strain of ftsZ AT . Since we were unable to construct a deletion of ftsZ AT , we used a depletion strategy in which ftsZ AT is present as a single copy under the control of an isopropyl β‐D‐1‐thiogalactopyranoside (IPTG) inducible promoter at a neutral site in the chromosome (Figueroa‐Cuilan et al ., ; Howell and Brown, ). Using western blot analysis, we have confirmed the depletion of FtsZ AT in the absence of IPTG (Supplemental Fig.…”

Section: Resultsmentioning

confidence: 98%

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Agrobacterium tumefaciens divisome proteins regulate the transition from polar growth to cell division

Howell

Aliashkevich

Sundararajan

et al. 2019

Molecular Microbiology

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Summary The mechanisms that restrict peptidoglycan biosynthesis to the pole during elongation and re‐direct peptidoglycan biosynthesis to mid‐cell during cell division in polar‐growing Alphaproteobacteria are largely unknown. Here, we explore the role of early division proteins of Agrobacterium tumefaciens including three FtsZ homologs, FtsA and FtsW in the transition from polar growth to mid‐cell growth and ultimately cell division. Although two of the three FtsZ homologs localize to mid‐cell, exhibit GTPase activity and form co‐polymers, only one, FtsZAT, is required for cell division. We find that FtsZAT is required not only for constriction and cell separation, but also for initiation of peptidoglycan synthesis at mid‐cell and cessation of polar peptidoglycan biosynthesis. Depletion of FtsZAT in A. tumefaciens causes a striking phenotype: cells are extensively branched and accumulate growth active poles through tip splitting events. When cell division is blocked at a later stage by depletion of FtsA or FtsW, polar growth is terminated and ectopic growth poles emerge from mid‐cell. Overall, this work suggests that A. tumefaciens FtsZ makes distinct contributions to the regulation of polar growth and cell division.

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Section: Resultssupporting

confidence: 62%

Section: Resultsmentioning

confidence: 98%

Agrobacterium tumefaciens divisome proteins regulate the transition from polar growth to cell division

Howell

Aliashkevich

Sundararajan

et al. 2019

Molecular Microbiology

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“…5F; see also Movie S5). The branching phenotype observed when pph was induced in A. tumefaciens cells is reminiscent of cells exhibiting a block in cell division (57)(58)(59)(60)(61)(62)(63). This observation suggests that PPH may have a dual function, namely, blocking cell division and triggering cell lysis.…”

Section: Phage Endolysin Triggers Lysis Of a Tumefaciensmentioning

confidence: 75%

“…The C terminus of PPH may have a similar function leading to the inhibition of a cell division protein. Indeed, A. tumefaciens cells expressing PPH exhibited a branching phenotype similar to that in FtsZ-depleted cells (63) (Fig. 5F; Movie S5).…”

Section: Phage Endolysin Triggers Lysis Of a Tumefaciensmentioning

confidence: 93%

“…See Table 3 for a list of all primers used in plasmid construction and sequencing. All variants of pph were cloned into the vector pSRKKm-Plac-sfgfp, which allows for inducible expression of target genes under the control of the lac promoter using IPTG as the inducer (63). To construct pSRKKm-PPH, PCR using Phusion high-fidelity DNA polymerase (Thermo Scientific) was performed on the Atu_ph02 genomic DNA using primers PPH NdeI F and PPH BamHI R. PCR products were gel purified using the GeneJET gel extraction kit (Thermo Scientific).…”

Section: Methodsmentioning

confidence: 99%

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Expression of a Peptidoglycan Hydrolase from Lytic Bacteriophages Atu_ph02 and Atu_ph03 Triggers Lysis of Agrobacterium tumefaciens

Attai

Rimbey

Smith

et al. 2017

Appl Environ Microbiol

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To provide food security, innovative approaches to preventing plant disease are currently being explored. Here, we demonstrate that lytic bacteriophages and phage lysis proteins are effective at triggering lysis of the phytopathogen Agrobacterium tumefaciens. Phages Atu_ph02 and Atu_ph03 were isolated from wastewater and induced lysis of C58-derived strains of A. tumefaciens. The coinoculation of A. tumefaciens with phages on potato discs limited tumor formation. The genomes of Atu_ph02 and Atu_ph03 are nearly identical and are ϳ42% identical to those of T7 supercluster phages. In silico attempts to find a canonical lysis cassette were unsuccessful; however, we found a putative phage peptidoglycan hydrolase (PPH), which contains a C-terminal transmembrane domain. Remarkably, the endogenous expression of pph in the absence of additional phage genes causes a block in cell division and subsequent lysis of A. tumefaciens cells. When the presumed active site of the N-acetylmuramidase domain carries an inactivating mutation, PPH expression causes extensive cell branching due to a block in cell division but does not trigger rapid cell lysis. In contrast, the mutation of positively charged residues at the extreme C terminus of PPH causes more rapid cell lysis. Together, these results suggest that PPH causes a block in cell division and triggers cell lysis through two distinct activities. Finally, the potent killing activity of this single lysis protein can be modulated, suggesting that it could be engineered to be an effective enzybiotic. IMPORTANCEThe characterization of bacteriophages such as Atu_ph02 and Atu_ph03, which infect plant pathogens such as Agrobacterium tumefaciens, may be the basis of new biocontrol strategies. First, cocktails of diverse bacteriophages could be used as a preventative measure to limit plant diseases caused by bacteria; a bacterial pathogen is unlikely to simultaneously develop resistances to multiple bacteriophage species. The specificity of bacteriophage treatment for the host is an asset in complex communities, such as in orchards where it would be detrimental to harm the symbiotic bacteria in the environment. Second, bacteriophages are potential sources of enzymes that efficiently lyse bacterial cells. These phage proteins may have a broad specificity, but since proteins do not replicate as phages do, their effect is highly localized, providing an alternative to traditional antibiotic treatments. Thus, studies of lytic bacteriophages that infect A. tumefaciens may provide insights for designing preventative strategies against bacterial pathogens.

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Programmable Gene Knockdown in Diverse Bacteria Using Mobile‐CRISPRi

et al. 2020

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Facile bacterial genome sequencing has unlocked a veritable treasure trove of novel genes awaiting functional exploration. To make the most of this opportunity requires powerful genetic tools that can target all genes in diverse bacteria. CRISPR interference (CRISPRi) is a programmable gene‐knockdown tool that uses an RNA‐protein complex comprised of a single guide RNA (sgRNA) and a catalytically inactive Cas9 nuclease (dCas9) to sterically block transcription of target genes. We previously developed a suite of modular CRISPRi systems that transfer by conjugation and integrate into the genomes of diverse bacteria, which we call Mobile‐CRISPRi. Here, we provide detailed protocols for the modification and transfer of Mobile‐CRISPRi vectors for the purpose of knocking down target genes in bacteria of interest. We further discuss strategies for optimizing Mobile‐CRISPRi knockdown, transfer, and integration. We cover the following basic protocols: sgRNA design, cloning new sgRNA spacers into Mobile‐CRISPRi vectors, Tn7 transfer of Mobile‐CRISPRi to Gram‐negative bacteria, and ICEBs1 transfer of Mobile‐CRISPRi to Bacillales. © 2020 The Authors. Basic Protocol 1: sgRNA design Basic Protocol 2: Cloning of new sgRNA spacers into Mobile‐CRISPRi vectors Basic Protocol 3: Tn7 transfer of Mobile‐CRISPRi to Gram‐negative bacteria Basic Protocol 4: ICEBs1 transfer of Mobile‐CRISPRi to Bacillales Support Protocol 1: Quantification of CRISPRi repression using fluorescent reporters Support Protocol 2: Testing for gene essentiality using CRISPRi spot assays on plates Support Protocol 3: Transformation of E. coli by electroporation Support Protocol 4: Transformation of CaCl2‐competent E. coli

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Mini-Tn 7 Insertion in an Artificial att Tn 7 Site Enables Depletion of the Essential Master Regulator CtrA in the Phytopathogen Agrobacterium tumefaciens

Cited by 45 publications

References 51 publications

Agrobacterium tumefaciens divisome proteins regulate the transition from polar growth to cell division

Agrobacterium tumefaciens divisome proteins regulate the transition from polar growth to cell division

Expression of a Peptidoglycan Hydrolase from Lytic Bacteriophages Atu_ph02 and Atu_ph03 Triggers Lysis of Agrobacterium tumefaciens

Programmable Gene Knockdown in Diverse Bacteria Using Mobile‐CRISPRi

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