PIGN spatiotemporally regulates the spindle assembly checkpoint proteins in leukemia transformation and progression

Author:

Teye Emmanuel K.,Lu Shasha,Chen Fangyuan,Yang Wenrui,Abraham Thomas,Stairs Douglas B.,Wang Hong-Gang,Yochum Gregory S.,Brodsky Robert A.,Pu Jeffrey J.

Abstract

AbstractPhosphatidylinositol glycan anchor biosynthesis class N (PIGN) has been linked to the suppression of chromosomal instability. The spindle assembly checkpoint complex is responsible for proper chromosome segregation during mitosis to prevent chromosomal instability. In this study, the novel role of PIGN as a regulator of the spindle assembly checkpoint was unveiled in leukemic patient cells and cell lines. Transient downregulation or ablation of PIGN resulted in impaired mitotic checkpoint activation due to the dysregulated expression of spindle assembly checkpoint-related proteins including MAD1, MAD2, BUBR1, and MPS1. Moreover, ectopic overexpression of PIGN restored the expression of MAD2. PIGN regulated the spindle assembly checkpoint by forming a complex with the spindle assembly checkpoint proteins MAD1, MAD2, and the mitotic kinase MPS1. Thus, PIGN could play a vital role in the spindle assembly checkpoint to suppress chromosomal instability associated with leukemic transformation and progression.

Funder

Aplastic Anemia and MDS International Foundation

American Cancer Society

NIDA/FDA

JTTai&Co Foundation Cancer Research Grant

Pennsylvania State University College of Medicine research grant

Publisher

Springer Science and Business Media LLC

Subject

Multidisciplinary

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