Susan Lovett

Susan Thomas Lovett
Susan Thomas Lovett
Born	Rochester, New York
Alma mater	Cornell University ; University of California, Berkeley
	Scientific career
Institutions	Brandeis University ; Lawrence Berkeley National Laboratory
Thesis	The recJ gene of Escherichia coli (1983)

Last updated January 01, 2022

Susan Thomas Lovett is an American molecular biologist who is the Abraham S. and Gertrude Burg Professor of Microbiology at Brandeis University. She is interested in the mechanisms that allow the genetic material in cells to remain stable over time.

Early life and education

Lovett was born in Rochester, New York.^[1] She spent her childhood in Virginia and Ohio.^[1] Lovett was an undergraduate student at Cornell University.^[2] She moved to the University of California, Berkeley for her doctoral research, where she investigated Escherichia coli .^[3] She was a postdoctoral researcher at Lawrence Berkeley National Laboratory.^[1]

Research and career

Lovett joined Brandeis University in 1989.^[4] She is a molecular biologist who studies the mechanisms that underpin DNA repair. In particular, Lovett has studied how cells protect their genetic information and avoid genetic mutation. These strategies help to tackle cancer and prevent cells from ageing. She has worked on the model organism Escherichia coli since the beginning of her career, and identified a secondary DNA damage response that is independent of the well-documented SOS response.^[5] Lovett identified many of the enzymes involves with DNA repair, including the post-transcriptional regulatory protein IraD, the ExoX and RecJ exonucleases, the Eubacterial protein RadA/Sms and the DNA helicase YoaA.^[5]

Amongst the repair mechanisms, Lovett has studied mutagenesis at the replication fork and how it coordinates with cellular cycles. She identified a GTPase proteins that couples cellular division with events at the replication fork. She has shown that chain-terminating drugs can be used, for example the AIDS drug, azidothymadine) to accumulate replication gaps, and that cellular nutrition impacts replication and repair.^[4]

Lovett has investigated the mutational hotspots that occur when strands of DNA do not align during the replication processes. Aberrant replication results in the rearrangement of DNA, which impacts the formation of mutational hotspots and exonuclease.^[6]

From 2006 to 2010, Lovett taught on the Cold Spring Harbor Laboratory course in Advanced Bacterial Genetics.^[1]

Awards and honors

2006 Elected Fellow of the American Society for Microbiology ^[2]
2008 Appointed to the Board of Directors of the Genetics Society of America ^[7]
2013 Elected Fellow of the American Association for the Advancement of Science ^[8]
2017 Brandeis University Dean of Arts and Sciences Service Award^[9]
2020 Elected Fellow of the American Academy of Arts and Sciences ^[4]
2021 Elected Fellow of the National Academy of Sciences ^[10]

Selected publications

Robert J Nichols; Saunak Sen; Yoe Jin Choo; et al. (23 December 2010). "Phenotypic landscape of a bacterial cell". Cell . 144 (1): 143–156. doi:10.1016/J.CELL.2010.11.052. ISSN 0092-8674. PMC 3060659 . PMID 21185072. Wikidata Q33780274.
S T Lovett; R D Kolodner (1 April 1989). "Identification and purification of a single-stranded-DNA-specific exonuclease encoded by the recJ gene of Escherichia coli". Proceedings of the National Academy of Sciences of the United States of America . 86 (8): 2627–2631. Bibcode:1989PNAS...86.2627L. doi:10.1073/PNAS.86.8.2627. ISSN 0027-8424. PMC 286970 . PMID 2649886. Wikidata Q33849909.
M Bzymek; S T Lovett (1 July 2001). "Instability of repetitive DNA sequences: the role of replication in multiple mechanisms". Proceedings of the National Academy of Sciences of the United States of America . 98 (15): 8319–8325. Bibcode:2001PNAS...98.8319B. doi:10.1073/PNAS.111008398. ISSN 0027-8424. PMC 37438 . PMID 11459970. Wikidata Q37096065.

Related Research Articles

A DNA polymerase is a member of a family of enzymes that catalyze the synthesis of DNA molecules from nucleoside triphosphates, the molecular precursors of DNA. These enzymes are essential for DNA replication and usually work in groups to create two identical DNA duplexes from a single original DNA duplex. During this process, DNA polymerase "reads" the existing DNA strands to create two new strands that match the existing ones. These enzymes catalyze the chemical reaction

A nuclease is an enzyme capable of cleaving the phosphodiester bonds between nucleotides of nucleic acids. Nucleases variously affect single and double stranded breaks in their target molecules. In living organisms, they are essential machinery for many aspects of DNA repair. Defects in certain nucleases can cause genetic instability or immunodeficiency. Nucleases are also extensively used in molecular cloning.

DNA polymerase I is an enzyme that participates in the process of prokaryotic DNA replication. Discovered by Arthur Kornberg in 1956, it was the first known DNA polymerase. It was initially characterized in E. coli and is ubiquitous in prokaryotes. In E. coli and many other bacteria, the gene that encodes Pol I is known as polA. The E. coli Pol I enzyme is composed of 928 amino acids, and is an example of a processive enzyme — it can sequentially catalyze multiple polymerisation steps without releasing the single-stranded template. The physiological function of Pol I is mainly to support repair of damaged DNA, but it also contributes to connecting Okazaki fragments by deleting RNA primers and replacing the ribonucleotides with DNA.

dnaQ is the gene encoding the ε subunit of DNA polymerase III in Escherichia coli. The ε subunit is one of three core proteins in the DNA polymerase complex. It functions as a 3’→5’ DNA directed proofreading exonuclease that removes incorrectly incorporated bases during replication. dnaQ may also be referred to as mutD.

The origin of replication is a particular sequence in a genome at which replication is initiated. Propagation of the genetic material between generations requires timely and accurate duplication of DNA by semiconservative replication prior to cell division to ensure each daughter cell receives the full complement of chromosomes. This can either involve the replication of DNA in living organisms such as prokaryotes and eukaryotes, or that of DNA or RNA in viruses, such as double-stranded RNA viruses. Synthesis of daughter strands starts at discrete sites, termed replication origins, and proceeds in a bidirectional manner until all genomic DNA is replicated. Despite the fundamental nature of these events, organisms have evolved surprisingly divergent strategies that control replication onset. Although the specific replication origin organization structure and recognition varies from species to species, some common characteristics are shared.

RecBCD is an enzyme of the E. coli bacterium that initiates recombinational repair from potentially lethal double strand breaks in DNA which may result from ionizing radiation, replication errors, endonucleases, oxidative damage, and a host of other factors. The RecBCD enzyme is both a helicase that unwinds, or separates the strands of DNA, and a nuclease that makes single-stranded nicks in DNA.

The nucleoid is an irregularly shaped region within the prokaryotic cell that contains all or most of the genetic material. The chromosome of a prokaryote is circular, and its length is very large compared to the cell dimensions, so it needs to be compacted in order to fit. In contrast to the nucleus of a eukaryotic cell, it is not surrounded by a nuclear membrane. Instead, the nucleoid forms by condensation and functional arrangement with the help of chromosomal architectural proteins and RNA molecules as well as DNA supercoiling. The length of a genome widely varies and a cell may contain multiple copies of it.

Stanley Norman Cohen is an American geneticist and the Kwoh-Ting Li Professor in the Stanford University School of Medicine. Stanley Cohen and Herbert Boyer were the first scientists to transplant genes from one living organism to another, a fundamental discovery for genetical engineering. Thousands of products have been developed on the basis of their work, including human growth hormone and hepatitis B vaccine. According to immunologist Hugh McDevitt, "Cohen's DNA cloning technology has helped biologists in virtually every field". Without it, "the face of biomedicine and biotechnology would look totally different."

DNA polymerase II is a prokaryotic DNA-Dependent DNA polymerase encoded by the PolB gene.

Prokaryotic DNA Replication is the process by which a prokaryote duplicates its DNA into another copy that is passed on to daughter cells. Although it is often studied in the model organism E. coli, other bacteria show many similarities. Replication is bi-directional and originates at a single origin of replication (OriC). It consists of three steps: Initiation, elongation, and termination.

Deoxyribonuclease IV (phage-T4-induced) is a kind of Endonuclease that catalyzes the degradation nucleotides in DsDNA by attacking the 5'-terminal end.

T7 DNA polymerase is an enzyme used during the DNA replication of the T7 bacteriophage. During this process, the DNA polymerase “reads” existing DNA strands and creates two new strands that match the existing ones. The T7 DNA polymerase requires a host factor, E. coli thioredoxin, in order to carry out its function. This helps stabilize the binding of the necessary protein to the primer-template to improve processivity by more than 100-fold, which is a feature unique to this enzyme. It is a member of the Family A DNA polymerases, which include E. coli DNA polymerase I and Taq DNA polymerase.

Thymineless death is the phenomenon by which bacteria, yeasts and mammalian cells undergo cell death when they are starved of thymidine triphosphate (dTTP), an essential precursor for DNA replication. This phenomenon underlies the mechanism of action of several antibacterial, antimalarial and anticancer agents, such as trimethoprim, sulfamethoxazole, methotrexate and fluorouracil.

Lorena Beese is a James B. Duke Professor of Biochemistry and Duke Cancer Institute Member. Her research involves structural mechanisms underlying DNA replication and repair, neurodegenerative diseases, cancer, and microbial pathogenesis; X-ray crystallography and cryo-electron microscopy; structure-based drug design; protein-protein and protein-nucleic acid interactions, enzyme mechanisms, chemical biology, protein structure and function.

DNA Polymerase V is a polymerase enzyme involved in DNA repair mechanisms in bacteria, such as Escherichia coli. It is composed of a UmuD' homodimer and a UmuC monomer, forming the UmuD'2C protein complex. It is part of the Y-family of DNA Polymerases, which are capable of performing DNA translesion synthesis (TLS). Translesion polymerases bypass DNA damage lesions during DNA replication - if a lesion is not repaired or bypassed the replication fork can stall and lead to cell death. However, Y polymerases have low sequence fidelity during replication. When the UmuC and UmuD' proteins were initially discovered in E. coli, they were thought to be agents that inhibit faithful DNA replication and caused DNA synthesis to have high mutation rates after exposure to UV-light. The polymerase function of Pol V was not discovered until the late 1990s when UmuC was successfully extracted, consequent experiments unequivocally proved UmuD'2C is a polymerase. This finding lead to the detection of many Pol V orthologs and the discovery of the Y-family of polymerases.

Ribonuclease T is a ribonuclease enzyme involved in the maturation of transfer RNA and ribosomal RNA in bacteria, as well as in DNA repair pathways. It is a member of the DnaQ family of exonucleases and non-processively acts on the 3' end of single-stranded nucleic acids. RNase T is capable of cleaving both DNA and RNA, with extreme sequence specificity discriminating against cytosine at the 3' end of the substrate.

Houra Merrikh is an Iranian-American microbiologist. She is a full professor at Vanderbilt University in the Department of Biochemistry. Her field of work is antibiotic resistance and bacterial evolvability.

Charles Clifton Richardson is an American biochemist and professor at Harvard University. Richardson received his undergraduate education at Duke University, where he majored in medicine. He received his M.D. at Duke Medical School in 1960. Richardson works as a professor at Harvard Medical School, and he served as editor/associate editor of the Annual Review of Biochemistry from 1972 to 2003. Richardson received the American Chemical Society Award in Biological Chemistry in 1968, as well as numerous other accolades.

Abraham Eisenstark was an American professor of microbiology. He was a Guggenheim Fellow for the academic year 1958–1959.

Elizabeth Lynn Zechiedrich is an American biochemist who is the Kyle and Josephine Morrow Chair in Molecular Virology and Microbiology at Baylor College of Medicine. Her research considers the structure-function properties of DNA and DNA topoisomerases. She was elected to the National Academy of Inventors in 2017.

References

1 2 3 4 "Susan T. Lovett". www.nasonline.org. Retrieved 2021-12-28.
1 2 "Susan Lovett | Brandeis University". www.brandeis.edu. Retrieved 2021-12-28.
↑ Lovett, Susan Thomas (1983). The recJ gene of Escherichia coli. OCLC 905884470.
1 2 3 "Professors Anita Hill and Susan Lovett elected to American Academy of Arts and Sciences". BrandeisNOW. Retrieved 2021-12-28.
1 2 "EcoSal Plus". EcoSal Plus. 2020. doi:10.1128/ecosalplus . Retrieved 2021-12-28.
↑ "Susan Lovett". www.brandeis.edu. Archived from the original on 2021-12-28. Retrieved 2021-12-28.
↑ "Genetics Society of America Announces 2011 Board Members". www.newswise.com. Archived from the original on 2021-12-28. Retrieved 2021-12-28.
↑ "AAAS Members Elected as Fellows | American Association for the Advancement of Science". www.aaas.org. Retrieved 2021-12-28.|archive-url= is malformed: timestamp (help)
↑ "School of Arts & Sciences Faculty Service Award". www.brandeis.edu. Retrieved 2021-12-28.|archive-url= is malformed: timestamp (help)
↑ "Susan Lovett elected to National Academy of Sciences". BrandeisNOW. Retrieved 2021-12-28.|archive-url= is malformed: timestamp (help)

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[:0-1] 1 2 3 4 "Susan T. Lovett". www.nasonline.org. Retrieved 2021-12-28.

[:1-2] 1 2 "Susan Lovett | Brandeis University". www.brandeis.edu. Retrieved 2021-12-28.

[3] Lovett, Susan Thomas (1983). The recJ gene of Escherichia coli. OCLC 905884470.

[:2-4] 1 2 3 "Professors Anita Hill and Susan Lovett elected to American Academy of Arts and Sciences". BrandeisNOW. Retrieved 2021-12-28.

[:3-5] 1 2 "EcoSal Plus". EcoSal Plus. 2020. doi:10.1128/ecosalplus . Retrieved 2021-12-28.

[6] "Susan Lovett". www.brandeis.edu. Archived from the original on 2021-12-28. Retrieved 2021-12-28.

[7] "Genetics Society of America Announces 2011 Board Members". www.newswise.com. Archived from the original on 2021-12-28. Retrieved 2021-12-28.

[8] "AAAS Members Elected as Fellows | American Association for the Advancement of Science". www.aaas.org. Retrieved 2021-12-28.|archive-url= is malformed: timestamp (help)

[9] "School of Arts & Sciences Faculty Service Award". www.brandeis.edu. Retrieved 2021-12-28.|archive-url= is malformed: timestamp (help)

[10] "Susan Lovett elected to National Academy of Sciences". BrandeisNOW. Retrieved 2021-12-28.|archive-url= is malformed: timestamp (help)

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