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Literature DB >> 30245083

Prospective Isolation and Characterization of Genetically and Functionally Distinct AML Subclones.

Bauke de Boer¹, Janine Prick¹, Maurien G Pruis¹, Peter Keane², Maria Rosaria Imperato², Jennifer Jaques¹, Annet Z Brouwers-Vos¹, Shanna M Hogeling¹, Carolien M Woolthuis¹, Marije T Nijk³, Arjan Diepstra⁴, Sebastian Wandinger⁵, Matthias Versele⁶, Ricardo M Attar⁶, Peter N Cockerill², Gerwin Huls¹, Edo Vellenga¹, André B Mulder³, Constanze Bonifer², Jan Jacob Schuringa⁷.

Abstract

Intra-tumor heterogeneity caused by clonal evolution is a major problem in cancer treatment. To address this problem, we performed label-free quantitative proteomics on primary acute myeloid leukemia (AML) samples. We identified 50 leukemia-enriched plasma membrane proteins enabling the prospective isolation of genetically distinct subclones from individual AML patients. Subclones differed in their regulatory phenotype, drug sensitivity, growth, and engraftment behavior, as determined by RNA sequencing, DNase I hypersensitive site mapping, transcription factor occupancy analysis, in vitro culture, and xenograft transplantation. Finally, we show that these markers can be used to identify and longitudinally track distinct leukemic clones in patients in routine diagnostics. Our study describes a strategy for a major improvement in stratifying cancer diagnosis and treatment. Crown

Entities: Disease Species

Keywords: DNase I hypersensitive site (DHS); FLT3-ITD; NRAS; WT1; acute myeloid leukemia (AML); clonal heterogeneity; digital footprinting; genetically distinct subclones; plasma membrane (PM); proteome

Mesh：

Substances：

Year: 2018 PMID： 30245083 DOI： 10.1016/j.ccell.2018.08.014

Source DB: PubMed Journal: Cancer Cell ISSN： 1535-6108 Impact factor: 31.743

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