Challenges and Advances in Genome Editing Technologies in Streptomyces

Zhao, Yawei; Li, Guoquan; Chen, Yunliang; Lü, Yinhua

doi:10.3390/biom10050734

“…In the conventional method, the derivatives of the target compounds were produced by the wild-type producer. Many strategies for genome editing of Streptomyces using CRISPR/Cas9 technology in vivo have been developed 37,38 ; however, it is still challenging to introduce a large DNA fragment into non-model host strains and to avoid off-targets especially in the PKS genes. In contrast, our approach is based on the high probability of heterologous expression in a versatile host.…”

Section: Resultsmentioning

confidence: 99%

In vitro Cas9-assisted editing of modular polyketide synthase genes to produce desired natural product derivatives

Kudo

¹

,

Hashimoto

²

,

Hashimoto

³

et al. 2020

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One major bottleneck in natural product drug development is derivatization, which is pivotal for fine tuning lead compounds. A promising solution is modifying the biosynthetic machineries of middle molecules such as macrolides. Although intense studies have established various methodologies for protein engineering of type I modular polyketide synthase(s) (PKSs), the accurate targeting of desired regions in the PKS gene is still challenging due to the high sequence similarity between its modules. Here, we report an innovative technique that adapts in vitro Cas9 reaction and Gibson assembly to edit a target region of the type I modular PKS gene. Proof-of-concept experiments using rapamycin PKS as a template show that heterologous expression of edited biosynthetic gene clusters produced almost all the desired derivatives. Our results are consistent with the promiscuity of modular PKS and thus, our technique will provide a platform to generate rationally designed natural product derivatives for future drug development.

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“…Significant developments in genetic engineering techniques can effectively help target and alter pathogenic bacterial genomes to recognize and mitigate drug resistance mechanisms. 188 , 189 The clustered regularly interspaced short palindromic repeats – CRISPR-associated (CRISPR-Cas) system, a bacterial adaptive immune system, is a newly recognized approach for controlling antibiotic-resistant strains, utilizing genomic engineering tools geared for gene knock-out and knock-in of sequence-specific DNA antibiotic targets. 189–191 The system is aimed to neutralize “the invasion by foreign genetic material” such as, bacteriophages, plasmids and transposons where the CRISPR-Cas9 acts as a “RNA-guided-DNA cutter”.…”

Section: The Way Forward: Protecting Global Healthmentioning

confidence: 99%

Antimicrobial Stewardship: Fighting Antimicrobial Resistance and Protecting Global Public Health

Majumder¹,

Rahman²,

Cohall³

et al. 2020

IDR

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“…Many strategies for genome editing of Streptomyces using CRISPR/Cas9 technology in vivo have been developed 37,38 ; however, it is still challenging to introduce a large DNA fragment into non-model host strains and to avoid off-targets especially in the PKS genes. In contrast, our approach is based on the high probability of heterologous expression in a versatile host.…”

Section: Discussionmentioning

confidence: 99%

Faculty Opinions recommendation of In vitro Cas9-assisted editing of modular polyketide synthase genes to produce desired natural product derivatives.

Awakawa

¹

2020

Faculty Opinions – Post-Publication Peer Review of the Biomedical Literature

0

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One major bottleneck in natural product drug development is derivatization, which is pivotal for fine tuning lead compounds. A promising solution is modifying the biosynthetic machineries of middle molecules such as macrolides. Although intense studies have established various methodologies for protein engineering of type I modular polyketide synthase(s) (PKSs), the accurate targeting of desired regions in the PKS gene is still challenging due to the high sequence similarity between its modules. Here, we report an innovative technique that adapts in vitro Cas9 reaction and Gibson assembly to edit a target region of the type I modular PKS gene. Proof-of-concept experiments using rapamycin PKS as a template show that heterologous expression of edited biosynthetic gene clusters produced almost all the desired derivatives. Our results are consistent with the promiscuity of modular PKS and thus, our technique will provide a platform to generate rationally designed natural product derivatives for future drug development.

show abstract

Challenges and Advances in Genome Editing Technologies in Streptomyces

Cited by 32 publications

References 78 publications

In vitro Cas9-assisted editing of modular polyketide synthase genes to produce desired natural product derivatives

In vitro Cas9-assisted editing of modular polyketide synthase genes to produce desired natural product derivatives

Antimicrobial Stewardship: Fighting Antimicrobial Resistance and Protecting Global Public Health

Faculty Opinions recommendation of In vitro Cas9-assisted editing of modular polyketide synthase genes to produce desired natural product derivatives.

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