Figure 5
Figure 5. Comparison of GP Ib, GP Ibα, and GP Ibβ from transfected CHO cells and human platelets. (A) GP Ib and GP Ibα from CHO cells and platelets of 2 donors (plt1, plt2) that had been resolved in a 5% Tris-glycine SDS gel under either nonreducing (N.R.) or reducing (R.) conditions and blotted by WM23. (B) GP Ibβ from CHO cells and platelets that had been resolved in a 4% to 12% Bis-Tris SDS gel under reducing (R.) conditions and blotted by Gi27. (C) Analysis of genomic Ibα gene sequences from the 2 donors. Genomic DNA was prepared from the buffy coat, and the VNTR-containing gene fragment was amplified by PCR along with various Ibα expression vectors. The amplified fragments were resolved in a 2.3% agarose gel. The 100 bp (base pair) DNA ladder was shown on the left. Four pcDNA-based vectors expressing GP Ibα with type A-D VNTR were included as standards on the right. (D) GP Ibα (type C VNTR) from platelets (plt2) and CHO cells before and after deglycosylation. Both Ibα were coimmunoprecipitated with SZ2 antibody, eluted from protein G-agarose beads, treated with a mixture of glycanases, resolved in a 5% Tris-glycine SDS gel under reducing conditions, and blotted by WM23.

Comparison of GP Ib, GP Ibα, and GP Ibβ from transfected CHO cells and human platelets. (A) GP Ib and GP Ibα from CHO cells and platelets of 2 donors (plt1, plt2) that had been resolved in a 5% Tris-glycine SDS gel under either nonreducing (N.R.) or reducing (R.) conditions and blotted by WM23. (B) GP Ibβ from CHO cells and platelets that had been resolved in a 4% to 12% Bis-Tris SDS gel under reducing (R.) conditions and blotted by Gi27. (C) Analysis of genomic Ibα gene sequences from the 2 donors. Genomic DNA was prepared from the buffy coat, and the VNTR-containing gene fragment was amplified by PCR along with various Ibα expression vectors. The amplified fragments were resolved in a 2.3% agarose gel. The 100 bp (base pair) DNA ladder was shown on the left. Four pcDNA-based vectors expressing GP Ibα with type A-D VNTR were included as standards on the right. (D) GP Ibα (type C VNTR) from platelets (plt2) and CHO cells before and after deglycosylation. Both Ibα were coimmunoprecipitated with SZ2 antibody, eluted from protein G-agarose beads, treated with a mixture of glycanases, resolved in a 5% Tris-glycine SDS gel under reducing conditions, and blotted by WM23.

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