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Dynamics of human telomerase recruitment depend on template-telomere base pairing. | LitMetric

Dynamics of human telomerase recruitment depend on template-telomere base pairing.

Mol Biol Cell

Howard Hughes Medical Institute and Department of Chemistry and Biochemistry, BioFrontiers Institute, University of Colorado Boulder, Boulder, CO 80309.

Published: April 2018

AI Article Synopsis

  • Telomerase is an enzyme that helps maintain chromosome stability by adding telomeric repeats, which counters telomere shortening in dividing human cells.
  • Researchers developed a live-cell imaging method to observe telomerase activity in CRISPR-edited HeLa cells, revealing how it interacts with chromosome ends.
  • Their findings indicate that telomerase's stable binding and its ability to efficiently add repeats are crucial for elongating telomeres, shedding light on its role in cancer cell biology.

Article Abstract

The reverse transcriptase telomerase adds telomeric repeats to chromosome ends to counteract telomere shortening and thereby assures genomic stability in dividing human cells. Key parameters in telomere homeostasis are the frequency with which telomerase engages the chromosome end and the number of telomeric repeats it adds during each association event. To study telomere elongation in vivo, we have established a live-cell imaging assay to track individual telomerase ribonucleoproteins in CRISPR-edited HeLa cells. Using this assay and the drug imetelstat, which is a competitive inhibitor of telomeric DNA binding, we demonstrate that stable association of telomerase with the single-stranded overhang of the chromosome end requires telomerase-DNA base pairing. Furthermore, we show that telomerase processivity contributes to telomere elongation in vivo. Together, these findings provide new insight into the dynamics of telomerase recruitment and the importance of processivity in maintaining telomere length in human cancer cells.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC5905299PMC
http://dx.doi.org/10.1091/mbc.E17-11-0637DOI Listing

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