Cavβ1 regulates T cell expansion and apoptosis independently of voltage-gated Ca2+ channel function

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作者
Serap Erdogmus
Axel R. Concepcion
Megumi Yamashita
Ikjot Sidhu
Anthony Y. Tao
Wenyi Li
Pedro P. Rocha
Bonnie Huang
Ralph Garippa
Boram Lee
Amy Lee
Johannes W. Hell
Richard S. Lewis
Murali Prakriya
Stefan Feske
机构
[1] Department of Pathology,Department of Pharmacology
[2] NYU Grossman School of Medicine,Unit on Genome Structure and Regulation
[3] Northwestern University,Department of Cancer Biology & Genetics
[4] National Institute of Child Health and Human Development,Department of Pharmacology
[5] National Institutes of Health,Department of Neuroscience
[6] National Cancer Institute,Department of Molecular and Cellular Physiology
[7] NIH,undefined
[8] National Institute of Allergy and Infectious Disease,undefined
[9] National Human Genome Research Institute,undefined
[10] Memorial Sloan Kettering Cancer Center,undefined
[11] University of California,undefined
[12] University of Texas-Austin,undefined
[13] Stanford University,undefined
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摘要
TCR stimulation triggers Ca2+ signals that are critical for T cell function and immunity. Several pore-forming α and auxiliary β subunits of voltage-gated Ca2+ channels (VGCC) were reported in T cells, but their mechanism of activation remains elusive and their contribution to Ca2+ signaling in T cells is controversial. We here identify CaVβ1, encoded by Cacnb1, as a regulator of T cell function. Cacnb1 deletion enhances apoptosis and impairs the clonal expansion of T cells after lymphocytic choriomeningitis virus (LCMV) infection. By contrast, Cacnb1 is dispensable for T cell proliferation, cytokine production and Ca2+ signaling. Using patch clamp electrophysiology and Ca2+ recordings, we are unable to detect voltage-gated Ca2+ currents or Ca2+ influx in human and mouse T cells upon depolarization with or without prior TCR stimulation. mRNAs of several VGCC α1 subunits are detectable in human (CaV3.3, CaV3.2) and mouse (CaV2.1) T cells, but they lack transcription of many 5’ exons, likely resulting in N-terminally truncated and non-functional proteins. Our findings demonstrate that although CaVβ1 regulates T cell function, these effects are independent of VGCC channel activity.
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