Transmitting genetic information without creating deleterious genetic alterations is one of the cell's most important tasks. Cells have evolved systems that check for and repair potentially lethal DNA damage. However, when these systems do not work properly, DNA damage accumulates and causes genetic changes or cell death. Accumulation of genetic changes, which is defined as a genomic instability is frequently observed in various types of genetic disorders including cancers. Genomic instability has been documented as a preceding step for multiple inactivations of tumor suppressor genes and activations of proto-oncogenes. One type of genomic instability observed frequently in many cancers is gross chromosomal rearrangement (GCR). GCR includes translocations, deletions of chromosome arm, interstitial deletions, inversions, amplifications, chromosome end-to-end fusion and aneuploidy. Although little is known about the origin and mechanisms of GCRs observed in cancer cells, recent studies on genes mutated in inherited cancer predisposition syndromes have started to demonstrate that proteins that function in DNA damage responses, DNA repair, and DNA recombination, play crucial roles in the suppression of spontaneous and/or DNA damage-induced GCRs. The recent identification of strong correlations between genes responsible for genetic diseases including cancers and GCRs started to pinpoint the importance of GCRs. However, the mechanisms that are responsible for GCR formation were not studied in depth. One of the major reasons for this is that many genes that suppress and enhance GCR formation have not yet been discovered. 1. Determine the role of RAD5 orthologs in mammalian GCR and further dissect the RAD5 pathway upstream signals and additional factors. Persistent stalled replication forks collapse and cause genomic instability that can lead to cell death if unrepaired. In yeast, stalled replication forks are resolved either by bypassing DNA damage with translesion synthesis (TLS) polymerases or by TS to the nascent strand of the sister chromatid. Different modifications of Proliferating Cell Nuclear Antigen (PCNA) determine the bypass mechanisms. PCNA functions to load different DNA polymerases or DNA repair machinery on DNA. PCNA is monoubiquitinated by RAD18 for damage bypass by TLS, and further poly-ubiquitinated by RAD5 on the monoubiquitinated PCNA for currently uncharacterized TS pathways. We found that yeast Rad18 and Rad5 suppress GCR through the poly-ubiquitination of PCNA. We recently demonstrated that mammals have RAD5-dependent TS pathway for suppression of genomic instability. There are two genes, SHPRH and HLTF, as RAD5 orthologs. We next hypothesized that mice deficient in SHPRH would show a high incidence of tumorigenesis. We have recently generated shprh-/- and hltf-/- and double knockout mice but did not observe tumorigenesis. In collaboration with Dr. Heinz Jacobs, we found that there is a redundant pathway that can complement the lack of SHPRH/HLTF pathway. We are currently searching for this complementary pathway. 2. ELG1: determine whether alternative Replication Factor C (RRFC) complex protein directs DNA repair pathways and communicates with cell cycle checkpoints. To investigate whether the role of ELG1 in GCR suppression is conserved in mammals, we cloned the human ELG1 gene by conducting a sequence homology search in the human genome database with help from the NHGRI Bioinformatics Core. When the expression of the human ELG1 gene was reduced by shRNA, an increase in DNA damage resulted as evidenced by an increase of phosphorylated histone H2Ax and ATM foci. The ELG1 protein was localized at the stalled replication fork after hydroxyurea treatment. We also demonstrated an increase of human ELG1 expression at S-phase and after treatment of cells with various DNA-damaging agents, including MMS, hydroxyurea, aphidicolin, and gamma-irradiation. We found that ELG1 interacts with PCNA and USP1 that removes ubiquitin from PCNA after TLS DNA damage bypass pathway. Based on these observations, we decided to investigate whether mice deficient in ELG1 would show a high incidence of tumorigenesis. In an attempt to create homozygous mice by using a retroviral insertion BayGenomics embryonic stem cell line, we found that the null mutation of mouse ELG1 is lethal at an early developmental stage. We confirmed this embryonic lethality in zebrafish model, too. To overcome this lethal event, we are continuing the last years effort to make a conditional knock out mouse model. Interestingly, we found that haploinsufficiency of ELG1 in mouse generated high incidence of tumors. In addition, in collaboration with Dr. Daphne Bell, we found human somatic mutations of ELG1 gene in many endometrial tumors. Lastly, since ELG1 protein level is increased in response to genotoxic stresses, we developed a robust assay to detect genotoxins. With this assay in collaboration with Drs. Christopher Austin, Menghang Xia, Raymond Tice, we screened 300,000 compounds collections in National Chemical Genomics Center to identify potential chemotherapeutic agents. We got 500 hit compounds. We are currently investigating potency of these compounds as chemotherapeutic agents. 3. Determine the role of Mph1, the yeast homolog of FANCM, in DNA repair By screening genes that enhance GCR formation when overexpressed, we identified MPH1 as the strongest GCR enhancing gene. MPH1 has been implicated in a homologous recombination (HR)-dependent DNA repair pathway. Recently, the human homolog of MPH1 was discovered as the gene mutated in FA complementation group M (FANCM) patients. FA is a genomic instability disorder clinically characterized by congenital abnormalities, progressive bone marrow failure, and predisposition to malignancy. The FA core complex consists of twelve proteins participating in a DNA damage response network with BRCA1 and BRCA2. FANCM is a recently identified component of the FA complex that is hypothesized to function at an early step of the FA pathway. MPH1 enhanced GCR formation when overexpressed. We hypothesized yeast has a FA like pathway. The first effort to identify more proteins functioning in this pathway, in collaboration with Dr. Weidong Wang, we found two proteins, MHF1 and MHF2 function in FA pathway in yeast as well as mammals. To make a yeast as an attractive model to study intercrosslink repair pathway that is a major pathway controlled by FA pathway, we studied genetic interactions of MPH1, MHF1, MHF2 and CHL1 with other DNA repair pathway. In this effort, we found yeast FA like pathway is regulated by RAD5-dependent TS pathway. We are currently investigating biochemical regulation of the yeast FA pathway by the RAD5 pathway.

Project Start
Project End
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Budget End
Support Year
9
Fiscal Year
2011
Total Cost
$1,300,592
Indirect Cost
Name
National Human Genome Research Institute
Department
Type
DUNS #
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