A major goal since the completion of the Human Genome Project has been to understand all functional elements in the human genome and the role they play in normal biological processes and disease. To that end, large pooled libraries of RNA interference (RNAi) reagents have been developed for genome-wide loss-of-function screens but have been hindered by 3 problems: 1) the incompleteness of protein depletion inherent in partial knock-down; 2) off-target effects from the seed sequence; and 3) genetic elements that are not transcribed are inaccessible to manipulation. Genome engineering using precisely targeted nucleases has emerged as an innovative technology to modify the genome and causally interrogate the role of different functional elements. Recently, I developed a new technology for functional genomic screening using the RNA- guided CRISPR/Cas9 nuclease (Shalem*, Sanjana*, et al., Science, 2014). Since CRISPR works on the DNA level, it is possible to manipulate non-coding elements that are inaccessible to RNAi. The research goal of this proposal is to develop new biological tools and analysis techniques for functional annotation of non-coding elements using pooled CRISPR screens. Mentored phase: First, I plan to develop and optimize high-throughput CRISPR non-coding mutagenesis libraries targeting introns, UTRs, promoters, non-coding RNAs, and intergenic regions to enable screening at high-resolution with megabase-scale coverage. Next, I will validate functional non-coding elements and use this large dataset to find unifying principles of how non-coding elements regulate gene expression. Independent phase: I plan to develop a novel CRISPR architecture for tiled deletion screens capable of deleting many segments over entire chromosomes or even entire genomes. With this technology and the increased screening throughput it enables, I will be able to develop a long-term independent research program in several possible directions, including further genome biology, personalized functional genomics, and predictive diagnostics for drug-genome interactions. The two primary areas of training needed to help me succeed in my research goals are 1) CRISPR technology development (mentor: Dr. Feng Zhang) and 2) knowledge of human genetics and non-coding variation (mentor: Dr. David Altshuler). Each mentor is an established expert in these fields. My career development plan integrates additional laboratory training, specialized tutorials in human genetics from world experts, local and national presentations of my research, and courses in scientific writing, grantsmanship and job search strategies. To assist with science- and career-related decisions, I have assembled an Advisory Committee with a team of established, senior genomics experts: Drs. Eric Lander, Steven Hyman, and David Root. The Broad Institute is an ideal environment: All Mentors and Advisors are located in one building and there are facilities for high-throughput functional screening in th RNAi Platform (Director: Dr. Root).

Public Health Relevance

This project seeks to transform our understanding of the human genome by developing a new kind of functional assay capable of directly editing the genome and analyzing how this genome editing impacts the growth, development, and drug resistance of human cells. The remarkable feature of this assay is its high capacity, which can test thousands of genome variations in a single experiment. This research will also improve our understanding of which parts of the genome are essential to life and which parts of the genome might be responsible for the proliferation of cancer cells.

Agency
National Institute of Health (NIH)
Institute
National Human Genome Research Institute (NHGRI)
Type
Career Transition Award (K99)
Project #
1K99HG008171-01
Application #
8804084
Study Section
National Human Genome Research Institute Initial Review Group (GNOM)
Program Officer
Pazin, Michael J
Project Start
2014-12-01
Project End
2016-11-30
Budget Start
2014-12-01
Budget End
2015-11-30
Support Year
1
Fiscal Year
2015
Total Cost
Indirect Cost
Name
Broad Institute, Inc.
Department
Type
DUNS #
623544785
City
Cambridge
State
MA
Country
United States
Zip Code
Sanjana, Neville E (2018) A genome-wide net to catch and understand cancer. Sci Transl Med 10:
Sanjana, Neville E (2017) Genome-scale CRISPR pooled screens. Anal Biochem 532:95-99
Jain, Isha H; Zazzeron, Luca; Goli, Rahul et al. (2016) Hypoxia as a therapy for mitochondrial disease. Science 352:54-61
Sanjana, Neville E; Wright, Jason; Zheng, Kaijie et al. (2016) High-resolution interrogation of functional elements in the noncoding genome. Science 353:1545-1549
Shalem, Ophir; Sanjana, Neville E; Zhang, Feng (2015) High-throughput functional genomics using CRISPR-Cas9. Nat Rev Genet 16:299-311
Canver, Matthew C; Smith, Elenoe C; Sher, Falak et al. (2015) BCL11A enhancer dissection by Cas9-mediated in situ saturating mutagenesis. Nature 527:192-7
Parnas, Oren; Jovanovic, Marko; Eisenhaure, Thomas M et al. (2015) A Genome-wide CRISPR Screen in Primary Immune Cells to Dissect Regulatory Networks. Cell 162:675-86
Chen, Sidi; Sanjana, Neville E; Zheng, Kaijie et al. (2015) Genome-wide CRISPR screen in a mouse model of tumor growth and metastasis. Cell 160:1246-60
Sanjana, Neville E; Shalem, Ophir; Zhang, Feng (2014) Improved vectors and genome-wide libraries for CRISPR screening. Nat Methods 11:783-784