Integrins are type I heterodimeric cell adhesion molecules that mediate a wide array of biological processes. Integrin bidirectional signaling allows communication between the cell interior with its microenvironment. The integrin transmembrane domains (TMs) are the transducers of activation signal that is relayed from the cytoplasmic domains to the distal ligand binding site located in the ectodomain of the integrin and vice versa. In this study, we showed that the disruption of the alpha L beta 2 TMs by mutation of a key interface residue Thr-686 in the beta 2 TM promoted alpha L beta 2 activation with ICAMs binding properties that are reminiscent of an intermediate affinity receptor. The activated alpha L beta 2 TM mutants, however, showed minimal reactivity with the reporter mAb KIM127 that recognizes a highly extended alpha L beta 2. Two models of alpha L beta 2 TM interaction were proposed previously. One with GXXXG-type interaction, and another that is based on TM cysteine-scanning analyses. Our data are consistent with a GXXXG-type interaction of the alpha L beta 2 TMs. Finally, we observed by FRET analyses that perturbation of the alpha L beta 2 TMs by beta 2 Thr-686 mutation facilitated alpha L microcluster formation. This was diminished by linking the alpha L beta 2 TMs with a disulfide bond, which served to clasp the TMs. These data suggest that disruption of the TM interface changes alpha L beta 2 ligand binding affinity, and it may contribute to alpha L micro-cluster formation.

• 出版日期2009-1-30
• 单位南阳理工学院