{"id":1730704,"date":"2025-06-17T11:14:50","date_gmt":"2025-06-17T15:14:50","guid":{"rendered":"https:\/\/med.virginia.edu\/faculty\/faculty-listing\/jlh2d\/"},"modified":"2025-06-25T15:12:01","modified_gmt":"2025-06-25T19:12:01","slug":"jlh2d","status":"publish","type":"faculty-listing","link":"https:\/\/med.virginia.edu\/faculty\/faculty-listing\/jlh2d\/","title":{"rendered":"Hamlin, Joyce L."},"content":{"rendered":"<p><b>Biochemistry, Molecular Biology, and Genetics<br \/>Cell and Developmental Biology<\/b><br \/>Our laboratory is interested in the control of mammalian chromosomal replication. It has been known for a long time that DNA replication initiates at multiple sites termed &quot;origins of replication&quot; along each DNA fiber. However, the precise location or properties of even a single origin had not been determined. Several years ago, we localized the first mammalian origin, which lies within the 55 kb spacer region between the DHFR and 2BE2121 genes. This spacer is characterized by the presence of a centered matrix attachment region (MAR). Using a two-dimensional gel electrophoretic technique to precisely identify initiation sites, we have shown that the origin corresponds to a very broad zone of potential sites scattered throughout the intergenic region. There are several genetic elements whose functions could contribute to the regulation of origin activity in this locus (e.g., a replicator, the promoters of the two flanking genes, the MAR). To identify the responsible controlling elements, we have devised a novel homologous recombination strategy to specifically knock out or mutagenize any fragment within the intergenic region or the two flanking genes. Our recent studies suggest that both the promoter and the 3&#8242; end of the DHFR gene are required for proper origin function. Surprisingly, however, the MAR is required to effect sister chromatid separation shortly after the origin fires. Our long-range goals are to define the initiation reaction in molecular terms by identifying both the cis- and trans-regulatory elements that participate, and to reconstitute initiation in vitro. <\/p>\n<p>To gain insight into whether the DHFR origin is typical of other mammalian   origins, we have recently devised a very efficacious strategy for isolating   all of the active origins in the human genome. The resulting library has been   shown to be essentially pure. By comparing the sequences of the origin clones   to the human genome database, we will be able to determine their distribrutions   vis-a-vis active genes, and whether or not they share common sequence motifs.   <br \/>  <b>Cancer Research &#8211; Molecular Medicine<\/b> <br \/>  We are interested in the mechanism by which cells amplify DNA. DNA sequence   amplification is an important phenomenon that only occurs in tumor cells, which   usually lack critical damage-sensing pathways. Most human tumors have amplified   one or more cellular oncogenes, which are thought to confer a selective growth   advantage over surrounding normal cells. Thus, it is important to determine   how gene amplification occurs. In fluorescence in situ hybridization studies,   we have shown that the very first amplification events are mediated by chromosome   breaks, followed by sister chromatid fusion, bridge formation, and further breaks.   Thus, it is now clear why cells that lack the ability to sense DNA damage (i.e.,   breaks) are able to amplify oncogenes, while normal cells cannot. We are devising   new strategies to examine the products of the earliest amplification events   at the nucleotide sequence level to determine why and how cell breaks and fusions   occur. Our goal is to identify steps in the amplification process that could   be targets for chemotherapy. <\/p>\n<p><b>Cell and Molecular Biology Training Program<\/b><br \/>  Our laboratory is interested in the control of mammalian chromosomal replication.   It has been known for a long time that DNA replication initiates at multiple   sites termed &quot;origins of replication&quot; along each DNA fiber. However,   the precise location or properties of even a single origin had not been determined.   Several years ago, we localized the first mammalian origin, which lies within   the 55 kb spacer region between the DHFR and 2BE2121 genes. This spacer is characterized   by the presence of a centered matrix attachment region (MAR). Using a two-dimensional   gel electrophoretic technique to precisely identify initiation sites, we have   shown that the origin corresponds to a very broad zone of potential sites scattered   throughout the intergenic region. There are several genetic elements whose functions   could contribute to the regulation of origin activity in this locus (e.g., a   replicator, the promoters of the two flanking genes, the MAR). To identify the   responsible controlling elements, we have devised a novel homologous recombination   strategy to specifically knock out or mutagenize any fragment within the intergenic   region or the two flanking genes. Our recent studies suggest that both the promoter   and the 3&#8242; end of the DHFR gene are required for proper origin function. Surprisingly,   however, the MAR is required to effect sister chromatid separation shortly after   the origin fires. Our long-range goals are to define the initiation reaction   in molecular terms by identifying both the cis- and trans-regulatory elements   that participate, and to reconstitute initiation in vitro. <\/p>\n<p>To gain insight into whether the DHFR origin is typical of other mammalian   origins, we have recently devised a very efficacious strategy for isolating   all of the active origins in the human genome. The resulting library has been   shown to be essentially pure. By comparing the sequences of the origin clones   to the human genome database, we will be able to determine their distribrutions   vis-a-vis active genes, and whether or not they share common sequence motifs.<\/p>\n<p>We are also interested in the mechanism by which cells amplify DNA. DNA sequence   amplification is an important phenomenon that only occurs in tumor cells, which   usually lack critical damage-sensing pathways. Most human tumors have amplified   one or more cellular oncogenes, which are thought to confer a selective growth   advantage over surrounding normal cells. Thus, it is important to determine   how gene amplification occurs. In fluorescence in situ hybridization studies,   we have shown that the very first amplification events are mediated by chromosome   breaks, followed by sister chromatid fusion, bridge formation, and further breaks.   Thus, it is now clear why cells that lack the ability to sense DNA damage (i.e.,   breaks) are able to amplify oncogenes, while normal cells cannot. We are devising   new strategies to examine the products of the earliest amplification events   at the nucleotide sequence level to determine why and how cell breaks and fusions   occur. Our goal is to identify steps in the amplification process that could   be targets for chemotherapy. <\/p>\n","protected":false},"featured_media":1734151,"template":"","meta":{"_acf_changed":false,"inline_featured_image":false,"_links_to":"","_links_to_target":""},"otheraff":[],"phd-degree":[],"primary":[2328],"research-discipline":[],"research-opportunity":[],"training-grant":[],"class_list":["post-1730704","faculty-listing","type-faculty-listing","status-publish","has-post-thumbnail","hentry","primary-biochemistry-and-molecular-genetics"],"acf":[],"yoast_head":"<!-- This site is optimized with the Yoast SEO plugin v27.4 - https:\/\/yoast.com\/product\/yoast-seo-wordpress\/ -->\n<title>Hamlin, Joyce L. - Research Faculty Directory<\/title>\n<meta name=\"robots\" content=\"index, follow, max-snippet:-1, max-image-preview:large, max-video-preview:-1\" \/>\n<link rel=\"canonical\" href=\"https:\/\/med.virginia.edu\/faculty\/faculty-listing\/jlh2d\/\" \/>\n<meta property=\"og:locale\" content=\"en_US\" \/>\n<meta property=\"og:type\" content=\"article\" \/>\n<meta property=\"og:title\" content=\"Hamlin, Joyce L. - Research Faculty Directory\" \/>\n<meta property=\"og:description\" content=\"Biochemistry, Molecular Biology, and GeneticsCell and Developmental BiologyOur laboratory is interested in the control of mammalian chromosomal replication. 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