Cooperation between Different CRISPR-Cas Types Enables Adaptation in an RNA-Targeting System

Ville Hoikkala; Janne Ravantti; César Díez-Villaseñor; Marja Tiirola; Rachel A Conrad; Mark J McBride; Sylvain Moineau; Lotta-Riina Sundberg

doi:10.1128/mBio.03338-20

Cooperation between Different CRISPR-Cas Types Enables Adaptation in an RNA-Targeting System

mBio. 2021 Mar 30;12(2):e03338-20. doi: 10.1128/mBio.03338-20.

Authors

Ville Hoikkala¹, Janne Ravantti², César Díez-Villaseñor¹, Marja Tiirola¹, Rachel A Conrad³, Mark J McBride³, Sylvain Moineau⁴, Lotta-Riina Sundberg⁵

Affiliations

¹ University of Jyväskylä Department of Biological and Environmental Science, Nanoscience Center, Jyväskylä, Finland.
² University of Helsinki, Molecular and Integrative Biosciences Research Programme, Helsinki, Finland.
³ University of Wisconsin-Milwaukee, Department of Biological Sciences, Milwaukee, Wisconsin, USA.
⁴ Université Laval, Département de Biochimie, de Microbiologie, et de Bio-informatique, Québec City, Québec, Canada.
⁵ University of Jyväskylä Department of Biological and Environmental Science, Nanoscience Center, Jyväskylä, Finland lotta-riina.sundberg@jyu.fi.

Abstract

CRISPR-Cas immune systems adapt to new threats by acquiring new spacers from invading nucleic acids such as phage genomes. However, some CRISPR-Cas loci lack genes necessary for spacer acquisition despite variation in spacer content between microbial strains. It has been suggested that such loci may use acquisition machinery from cooccurring CRISPR-Cas systems within the same strain. Here, following infection by a virulent phage with a double-stranded DNA (dsDNA) genome, we observed spacer acquisition in the native host Flavobacterium columnare that carries an acquisition-deficient CRISPR-Cas subtype VI-B system and a complete subtype II-C system. We show that the VI-B locus acquires spacers from both the bacterial and phage genomes, while the newly acquired II-C spacers mainly target the viral genome. Both loci preferably target the terminal end of the phage genome, with priming-like patterns around a preexisting II-C protospacer. Through gene deletion, we show that the RNA-cleaving VI-B system acquires spacers in trans using acquisition machinery from the DNA-cleaving II-C system. Our observations support the concept of cross talk between CRISPR-Cas systems and raise further questions regarding the plasticity of adaptation modules.IMPORTANCE CRISPR-Cas systems are immune systems that protect bacteria and archaea against their viruses, bacteriophages. Immunity is achieved through the acquisition of short DNA fragments from the viral invader's genome. These fragments, called spacers, are integrated into a memory bank on the bacterial genome called the CRISPR array. The spacers allow for the recognition of the same invader upon subsequent infection. Most CRISPR-Cas systems target DNA, but recently, systems that exclusively target RNA have been discovered. RNA-targeting CRISPR-Cas systems often lack genes necessary for spacer acquisition, and it is thus unknown how new spacers are acquired and if they can be acquired from DNA phages. Here, we show that an RNA-targeting system "borrows" acquisition machinery from another CRISPR-Cas locus in the genome. Most new spacers in this locus are unable to target phage mRNA and are therefore likely redundant. Our results reveal collaboration between distinct CRISPR-Cas types and raise further questions on how other CRISPR-Cas loci may cooperate.

Keywords: CRISPR; adaptation; bacteriophages; coevolution; spacer acquisition; type II; type VI.

Publication types

Research Support, Non-U.S. Gov't
Research Support, U.S. Gov't, Non-P.H.S.

MeSH terms

Adaptation, Physiological
Bacteriophages / genetics*
Bacteriophages / physiology
CRISPR-Cas Systems*
Clustered Regularly Interspaced Short Palindromic Repeats
Flavobacterium / genetics*
Flavobacterium / physiology
Flavobacterium / virology*
Genome, Bacterial
RNA, Viral / genetics
RNA, Viral / metabolism*

Substances

RNA, Viral

Supplementary concepts

Flavobacterium columnare