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Rockefeller University

Luciano Marraffini, Ph.D.

Kayden Family Professor
Investigator, Howard Hughes Medical Institute

Investigates how CRISPR-Cas systems provide adaptive immunity to bacteria.

CRISPR-Cas systems enable bacteria to acquire immunity against their viruses by capturing snippets of their DNA and using RNA-guided nucleases that cleave the viral DNA. Marraffini investigates the molecular mechanisms that make CRISPR immunity possible, and also explores genome editing and other potential applications for CRISPR-Cas systems.

Sequence-directed genetic interference pathways control gene expression and preserve genome integrity in all kingdoms of life. In bacteria and archaea, CRISPRs—clustered, regularly interspaced, short palindromic repeats—constitutes a recently discovered genetic interference pathway that protects cells from phages and conjugative plasmids. Within CRISPR sites, the repeats are separated by short spacer sequences that match phage or plasmid genomes and specify the targets of interference.

Spacer sequences are transcribed into CRISPR RNAs (crRNAs)—small RNAs that, through base-pairing interactions with the target sequence, guide Cas nucleases to the invasive nucleic acid to cleave it. Upon infection, CRISPR arrays can acquire new spacer units that match the sequence of the infecting phage or plasmid. In this way, CRISPR-Cas systems provide adaptive and inheritable immunity to the bacterial cell. The spacer content of CRISPR arrays reflects the many different invaders encountered by the host and can be expanded rapidly in response to new ones. Accordingly, CRISPR loci constitute a form of genetic memory that ensures the rejection of new, returning, and ever-present invading DNA molecules.

Marraffini uses Staphylococcus epidermidis and Streptococcus pyogenes as model systems for studying CRISPR immunity. The clinical isolate S. epidermidis RP62a harbors a CRISPR spacer that matches the nickase gene (nes) that is present in nearly all staphylococcal conjugative plasmids and prevents their spread. Using this system, he revealed that the CRISPR-Cas machinery targets DNA, rather than RNA, directly. Work in the Marraffini lab also demonstrated that the S. pyogenes crRNA-guided Cas9 DNA nuclease constitute a formidable tool for genetic engineering.

His current research employs molecular genetic and biochemical approaches to analyze the function of CRISPR-Cas systems. Marraffini ultimately hopes to answer fundamental questions about how CRISPR-Cas systems destroy their targets, how the genetic memory is generated, and how CRISPR-Cas immunity affects the evolution of bacteria and archaea.

Marraffini is a faculty member in the David Rockefeller Graduate Program, the Tri-Institutional M.D.-Ph.D. Program, and the Tri-Institutional Ph.D. Program in Chemical Biology.

Education

Lic. in biotechnology, 1998
University of Rosario

Ph.D. in microbiology, 2007
University of Chicago

Postdoc

Northwestern University, 2008–2010

Positions

Assistant Professor, 2010–2016
Associate Professor 2016–2018
Professor, 2018–
The Rockefeller University

Investigator, 2018–
Howard Hughes Medical Institute

Awards

RNA Society Award, 2010

Searle Scholar, 2011

Rita Allen Foundation Scholar, 2012

NIH Director’s New Innovator Award, 2012

The Rockefeller University Distinguished Teaching Award, 2013

40 Under 40, Cell, 2014

Hans Sigrist Prize, 2015

Earl and Thressa Stadtman Scholar Award, 2016

Howard Hughes Medical Institute Faculty Scholar, 2016

Albany Medical Center Prize in Medicine and Biomedical Research, 2017

Gabrielle H. Reem and Herbert J. Kayden Early-Career Innovation Award, 2017

NIH Director’s Pioneer Award, 2017

Max Planck-Humboldt Medal, 2020

Genetics Society of America Medal, 2024

Vilcek Prize in Biomedical Science, 2024

Honorary Societies

National Academy of Sciences

American Academy of Microbiology

American Academy of Arts and Sciences

Selected Publications

Maguin, P. et al. Cleavage of viral DNA by restriction endonucleases stimulates the type II CRISPR-Cas immune response. Molecular Cell 82, 907–919 (2022).

Mo, C.Y. et al. Type III-A CRISPR immunity promotes mutagenesis of staphylococci. Nature 592, 611–615 (2021).

Meeske, A.J. et al. A phage-encoded anti-CRISPR enables complete evasion of type VI-A CRISPR-Cas immunity. Science 369, 54–59 (2020).

Modell, J.W. et al. CRISPR-Cas systems exploit viral DNA injection to establish and maintain adaptive immunity. Nature 544, 101–104 (2017).

Jiang, W. et al. Degradation of phage transcripts by CRISPR-associated RNases enables type III CRISPR-Cas immunity. Cell 164, 710–721 (2016).

Additional Links

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