4.7 Article

Identifying C. elegans lifespan mutants by screening for early-onset protein aggregation

期刊

ISCIENCE
卷 25, 期 11, 页码 -

出版社

CELL PRESS
DOI: 10.1016/j.isci.2022.105460

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资金

  1. NIH Office of Research Infrastructure Pro-grams
  2. U.S. National Institutes of Health (NIH)
  3. [P40 OD010440]
  4. [R00AG046911]
  5. [R21AG059099]

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In this study, we used microfluidic technologies and image processing to perform high-throughput automated screening for short-lived mutants based on protein aggregation. We identified lifespan mutants by screening for accelerated protein aggregation through quantitative analysis of fluorescently labeled aggregates, avoiding the need for conditional sterilization or manual separation.
Genetic screens are widely used to identify genes that control specific biological functions. In Caenorhabditis elegans, forward genetic screens rely on the isolation of reproductively active mutants that can self-propagate clonal populations. Screens that target post-reproductive phenotypes, such as lifespan, are thus challenging. We combine microfluidic technologies and image processing to perform high-throughput automated screening for short-lived mutants using protein aggregation as a marker for aging. We take advantage of microfluidics for maintaining a reproductively active adult mutagenized population and for performing serial high-throughput analysis and sorting of animals with increased protein aggregation, using fluorescently-labeled PAB-1 as a readout. We demonstrate that lifespan mutants can be identified by screening for accelerated protein aggregation through quantitative analysis of fluorescently labeled aggregates while avoiding conditional sterilization or manual separation of parental and progeny populations. We also show that aged wildtypes and premature aggregation mutants differ in aggregate morphology, suggesting aggregate growth is time-dependent.

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