cated efficiently into the ER in sec61L7 cells, and when we blott

cated efficiently into the ER in sec61L7 cells, and when we blotted on wildtype and mutant extracts we did not detect cytosolic BiP precur sor in sec61L7 cells. ERAD of KHN, how ever, was strongly defective in the sec61L7 mutant in contrast to ERAD of its membrane anchored counterpart KWW whose half life increased only moderately. BAY 73-4506 Since KHN and KWW have been shown by Vashist and Ng to have identical chaperone requirements for ERAD, this experiment demonstrates that rather than affecting indirectly the chaperone composition in the ER lumen sec61L7 has a direct negative effect on export from the ER of soluble substrates only. The sec61Y345H mutant had no growth defect at any temperature, and a tunicamycin sensitivity comparable to sec61 32 and sec61 3.

It was fully functional in protein import into the ER suggesting that this position in L7 might play a role in the initiation of Sec61 channel opening from the lumenal side for ex port of ERAD substrates. One would expect a mild phenotype in order for mice to survive this mutation in an essential gene. Delayed ER export in pancreatic beta cells which have a high secretory protein load would result in gradual ER accumulation of misfolded proteins, followed by cell death, and the development of diabetes as a primary phenotype. The delay in the initiation of ERAD in sec61Y345H yeast is reminiscent of the delay in protein import observed by Trueman et al. in L7 mutants that disrupt the interaction of L7 with TMD7. Taken together, our data suggest that L7 conformation is crucial for Sec61 channel gating for both import and ERAD of soluble proteins.

Modelling of the Sec61L7 protein suggests that the plug formed by transmembrane helix 2a remains in place, but the lateral gate formed by interaction of trans membrane helix 2b with transmembrane helix 7 is par tially open, as helix 2b is shifted significantly towards the cytoplasmic surface of the membrane. This shift is likely the consequence of the missing lumenal end of TMD7 which can no longer interact with helix 2b and hold it in place. The deletion in Sec61L7p begins 2 amino acids C terminal of N302 which is the most C terminal residue of the gating motif responsible for setting the hydrophobicity threshold for entry of signal sequences into the Sec61 channel. Destabilizing the gating motif by replacing N302 with more polar amino acids causes promiscuous insertion of even marginally hydrophobic signal peptides into the gate.

In SecL7p N302 is under strain because it is now close to the end of trun cated TMD7 which is connected to TMD8 by only 2 amino acids. This will weaken the hydrogen bonds to N302 partners in AV-951 the gating motif which likely explains the partial opening of the gate. While selleckchem Crizotinib the destabilization of the lateral gate in the Sec61L7 channel is similar to that of the N302 to polar mutants, in contrast to Trueman et al. we do not see enhanced import of soluble proteins by the Sec61L7 channel, but rather an almost complete block of transport of so

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