![Figure 1. Blocking of integrin β1 and β3 inhibits adhesion to α3(IV)NC1 domain. (A) Cell adhesion assay. MLECs were seeded onto a 96-well plate coated with α3(IV)NC1 in the presence of the indicated integrin antibodies and cell adhesion was evaluated. Values are means (± the standard error of the mean [SEM]) of triplicate wells. Differences between 3 independent experiments control IgG and various integrin antibodies treated cells binding were significant. *P < .05 and **P < .01. (B) Proliferation assay. Similar to panel A, cells were preincubated with indicated integrin proteins with and without α3(IV)NC1 and cell proliferation was evaluated. The results are shown as mean (± the standard error of the mean [SEM]) *P < .05, α3(IV)NC1 without vs with α3β1 and αVβ3 integrins. **P < .008, α3(IV)NC1 without vs with α3β1 + αVβ3 integrins together. (C-I) Identification of α3(IV)NC1 functional binding integrins. MLECs were treated with α3(IV)NC1 for approximately 6 hours and extracts were immunoprecipitated with anti-α3(IV)NC1 antibody or control IgG. Immunoprecipitates were fractionated by SDS-PAGE and immunoblotted with anti-α3(IV)NC1, αV, α3, β3, β1, α1, and α5 antibodies. Crude cell lysate was used as a positive control.](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/110/4/10.1182_blood-2007-01-066282/5/zh80140704970001.jpeg?Expires=1723447490&Signature=gvEs8Tl8Du5fiFl-d9kX8sRGxvICDGh9busPvQ~cMkv69jirgaDTxhUy5Uzkr7Qcf4Lhcqz52-hxiC9qEbCqS4FiFka2PbvjJ9YU7kv-xfDdgj879dLfksVp17Uso6Uvi4VJPQnJOfipV77SG4Nc2LCsk4G9ayuwGLVrcKV2C1C1RoBSvJuiubY8QoXB8VR40SoBey5Khq3ou7VpGY62h3xkEfWXTHs3XXMotnDb-If0bZ5YZy45TZ9VniHfOLZemeOsp1NwAbsHIXJR0Aqvf2yteiqTtvsWEsrQMnGOJkEI3Wo2lA1GPQUE94ImWIrE0afUhEW49l-7XPPY97gOiA__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
Blocking of integrin β1 and β3 inhibits adhesion to α3(IV)NC1 domain. (A) Cell adhesion assay. MLECs were seeded onto a 96-well plate coated with α3(IV)NC1 in the presence of the indicated integrin antibodies and cell adhesion was evaluated. Values are means (± the standard error of the mean [SEM]) of triplicate wells. Differences between 3 independent experiments control IgG and various integrin antibodies treated cells binding were significant. *P < .05 and **P < .01. (B) Proliferation assay. Similar to panel A, cells were preincubated with indicated integrin proteins with and without α3(IV)NC1 and cell proliferation was evaluated. The results are shown as mean (± the standard error of the mean [SEM]) *P < .05, α3(IV)NC1 without vs with α3β1 and αVβ3 integrins. **P < .008, α3(IV)NC1 without vs with α3β1 + αVβ3 integrins together. (C-I) Identification of α3(IV)NC1 functional binding integrins. MLECs were treated with α3(IV)NC1 for approximately 6 hours and extracts were immunoprecipitated with anti-α3(IV)NC1 antibody or control IgG. Immunoprecipitates were fractionated by SDS-PAGE and immunoblotted with anti-α3(IV)NC1, αV, α3, β3, β1, α1, and α5 antibodies. Crude cell lysate was used as a positive control.
