Journal
CELL
Volume 171, Issue 2, Pages 321-+Publisher
CELL PRESS
DOI: 10.1016/j.cell.2017.09.004
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Categories
Funding
- California Institute for Regenerative Medicine [GC1R-06673]
- Center of Excellence for Stem Cell Genomics
- NIH [U01-HL099999, U01-HL099995, UC4DK104211, DK10261201, P30DK116074-01]
- Helmsley Charitable Trust
- H.L. Snyder Foundation
- Elser Foundation
- JDRF
- Wallenberg Research link at Stanford University [KAW 2013.0391]
- JDRF [3-APF-2016-172-A-N]
- NIDDK [5T32DK007217-39]
- Swedish Research Council [2015-00599]
- Swedish Research Council [2015-00599] Funding Source: Swedish Research Council
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As organisms age, cells accumulate genetic and epigenetic errors that eventually lead to impaired organ function or catastrophic transformation such as cancer. Because aging reflects a stochastic process of increasing disorder, cells in an organ will be individually affected in different ways, thus rendering bulk analyses of postmitotic adult cells difficult to interpret. Here, we directly measure the effects of aging in human tissue by performing single-cell transcriptome analysis of 2,544 human pancreas cells from eight donors spanning six decades of life. We find that islet endocrine cells from older donors display increased levels of transcriptional noise and potential fate drift. By determining the mutational history of individual cells, we uncover a novel mutational signature in healthy aging endocrine cells. Our results demonstrate the feasibility of using single-cell RNA sequencing (RNA-seq) data from primary cells to derive insights into genetic and transcriptional processes that operate on aging human tissue.
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