Lamin B1 and LAP2ß resist cytoskeletal force to maintain lamin A/C meshwork organization and preserve nuclear integrity

The nuclear lamins are extremely long-lived proteins in most cell types. As a consequence, lamin function cannot be effectively dissected with temporal precision using standard knock-down approaches. Here, we apply the auxin inducible degron (AID) system to rapidly deplete each lamin isoform within one cell cycle and reveal the immediate impacts of lamin loss on the nucleus . Surprisingly, neither acute lamin A/C (LA/C), lamin B1 (LB1), nor lamin B2 (LB2) depletion altered nuclear shape or induced nuclear blebbing, indicating that acute lamin loss is not sufficient to alter nuclear morphology. LB1 depletion is immediately followed by LA/C meshwork disorganization due to actin cytoskeletal forces on the lamina, yet neither LA/C nor LB1 depletion induced nuclear rupturing. We found that the abundant inner nuclear membrane protein LAP2ß protects nuclear integrity in the absence of LB1, as depletion of both LB1 and LAP2ß induced severe LA/C disorganization and frequent nuclear rupturing. Depolymerization of the actin cytoskeleton halts nuclear rupture in LAP2ß- and LB1-depleted nuclei. We conclude that both LB1 and LAP2ß resist cytoskeletal force to maintain regular lamin A/C meshwork organization and preserve nuclear integrity. Overall design: RNA-seq profiling of DLD1 cells expressing Lamin A/C, Lamin B1 or Lamin B2 endogenously tagged with an N-terminal auxin inducible degron tag. Cells were treated with auxin for 0, 16, or 96 hours. Non-tagged DLD1 parental cells were also treated with auxin for 0, 16, or 96 hours to generate a list of auxin responsive genes.