Long non-coding RNA-dependent mechanism to regulate heme biosynthesis and erythrocyte development

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作者
Jinhua Liu
Yapu Li
Jingyuan Tong
Jie Gao
Qing Guo
Lingling Zhang
Bingrui Wang
Hui Zhao
Hongtao Wang
Erlie Jiang
Ryo Kurita
Yukio Nakamura
Osamu Tanabe
James Douglas Engel
Emery H. Bresnick
Jiaxi Zhou
Lihong Shi
机构
[1] State Key Laboratory of Experimental Hematology,Tianjin Key Laboratory of Food and Biotechnology, School of Biotechnology and Food Science
[2] Institute of Hematology and Blood Diseases Hospital,Department of Integrative Genomics Tohoku Medical Megabank
[3] Chinese Academy of Medical Sciences & Peking Union Medical College,Department of Cell and Developmental Biology
[4] Center for Stem Cell Medicine,Wisconsin Institutes for Medical Research, Paul Carbone Cancer Center, Department of Cell and Regenerative Biology
[5] Chinese Academy of Medical Sciences,undefined
[6] Tianjin University of Commerce,undefined
[7] Japanese Red Cross Society,undefined
[8] Department of Research and Development,undefined
[9] Central Blood Institute,undefined
[10] RIKEN BioResource Research Center,undefined
[11] Cell Engineering Division,undefined
[12] Tohoku University,undefined
[13] University of Michigan Medical School,undefined
[14] University of Wisconsin School of Medicine and Public Health,undefined
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摘要
In addition to serving as a prosthetic group for enzymes and a hemoglobin structural component, heme is a crucial homeostatic regulator of erythroid cell development and function. While lncRNAs modulate diverse physiological and pathological cellular processes, their involvement in heme-dependent mechanisms is largely unexplored. In this study, we elucidated a lncRNA (UCA1)-mediated mechanism that regulates heme metabolism in human erythroid cells. We discovered that UCA1 expression is dynamically regulated during human erythroid maturation, with a maximal expression in proerythroblasts. UCA1 depletion predominantly impairs heme biosynthesis and arrests erythroid differentiation at the proerythroblast stage. Mechanistic analysis revealed that UCA1 physically interacts with the RNA-binding protein PTBP1, and UCA1 functions as an RNA scaffold to recruit PTBP1 to ALAS2 mRNA, which stabilizes ALAS2 mRNA. These results define a lncRNA-mediated posttranscriptional mechanism that provides a new dimension into how the fundamental heme biosynthetic process is regulated as a determinant of erythrocyte development.
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