| Literature DB >> 31000603 |
Hongsheng Wang1, Shweta Jain2, Peng Li3,4, Jian-Xin Lin3,4, Jangsuk Oh3,4, Chenfeng Qi2, Yuanyuan Gao2, Jiafang Sun2, Tomomi Sakai2, Zohreh Naghashfar2, Sadia Abbasi2, Alexander L Kovalchuk2, Silvia Bolland2, Stephen L Nutt5,6, Warren J Leonard7,4, Herbert C Morse1.
Abstract
The IRF and Ets families of transcription factors regulate the expression of a range of genes involved in immune cell development and function. However, the understanding of the molecular mechanisms of each family member has been limited due to their redundancy and broad effects on multiple lineages of cells. Here, we report that double deletion of floxed Irf8 and Spi1 (encoding PU.1) by Mb1-Cre (designated DKO mice) in the B cell lineage resulted in severe defects in the development of follicular and germinal center (GC) B cells. Class-switch recombination and antibody affinity maturation were also compromised in DKO mice. RNA-seq (sequencing) and ChIP-seq analyses revealed distinct IRF8 and PU.1 target genes in follicular and activated B cells. DKO B cells had diminished expression of target genes vital for maintaining follicular B cell identity and GC development. Moreover, our findings reveal that expression of B-cell lymphoma protein 6 (BCL6), which is critical for development of germinal center B cells, is dependent on IRF8 and PU.1 in vivo, providing a mechanism for the critical role for IRF8 and PU.1 in the development of GC B cells.Entities:
Keywords: BCL6; IRF8; PU.1; follicular B cells; germinal center
Year: 2019 PMID: 31000603 PMCID: PMC6511064 DOI: 10.1073/pnas.1901258116
Source DB: PubMed Journal: Proc Natl Acad Sci U S A ISSN: 0027-8424 Impact factor: 11.205