Figure 7
Figure 7. Binding of ERp5 and ERp5-AGHA to αIIbβ3 and directly to the β3 subunit. (A) Binding of αIIbβ3 to immobilized ERp5 or ERp5-AGHA was measured in the presence or absence of MnCl2 (Mn++; 2 mM), in the presence of EDTA (5 mM), or in the absence of added αIIbβ3 (background), as indicated. Bound αIIbβ3 was detected with an anti-CD41 conformation-independent antibody. ERp5 (black) and ERp5-AGHA (gray) binding to αIIbβ3 were compared by nonparametric Student t tests: no Mn++ vs Mn++ and no Mn++ vs background,***P < .0001. There is no significant difference between no Mn++ vs EDTA. Results are the average of 3 experiments. (B) Binding of ERp5 (100 nM) or ERp5-AGHA (100 nM) to αIIbβ3 (black) or glycoprotein (GP)Ibα (gray), both coated at 20 nM on 96-well plates in the absence of Mn++ or in the absence of bound ERp5 or ERp5-AGHA (background; white). Bound ERp5 or ERp5-AGHA was detected with anti-ERp5 antibody. ERp5 binding to αIIbβ3 vs GPIba, ERp5-AGHA binding to αIIbβ3 vs GPIbα, ERp5 binding to αIIbβ3 vs background, and ERp5-AGHA binding to αIIbβ3 vs background, **P < .005. Binding of ERp5 or ERp5-AGHA to GPIbα vs background was not statistically significant. Results are the average of 3 experiments. Surface plasmon resonance was used to determine the binding constant for ERp5 with recombinant β3 integrin tagged with calmodulin in the presence (C) or absence of Mn++ (D). ERp5 was coated on the Biacore chip. Lines represent the fitted curves of ERp5 at concentrations of 0, 0.33, 0.66, 1.31, 2.63, 5.25, 10.25, 21, and 42 µM. The KD values for ERp5 interaction with the β3 subunit in the presence and absence of Mn++ were 21.7 μM and 19.1 μM, respectively. ERp5 did not bind to calmodulin alone. n.s., not significant; RU, relative units.

Binding of ERp5 and ERp5-AGHA to αIIbβ3 and directly to the β3 subunit. (A) Binding of αIIbβ3 to immobilized ERp5 or ERp5-AGHA was measured in the presence or absence of MnCl2 (Mn++; 2 mM), in the presence of EDTA (5 mM), or in the absence of added αIIbβ3 (background), as indicated. Bound αIIbβ3 was detected with an anti-CD41 conformation-independent antibody. ERp5 (black) and ERp5-AGHA (gray) binding to αIIbβ3 were compared by nonparametric Student t tests: no Mn++ vs Mn++ and no Mn++ vs background,***P < .0001. There is no significant difference between no Mn++ vs EDTA. Results are the average of 3 experiments. (B) Binding of ERp5 (100 nM) or ERp5-AGHA (100 nM) to αIIbβ3 (black) or glycoprotein (GP)Ibα (gray), both coated at 20 nM on 96-well plates in the absence of Mn++ or in the absence of bound ERp5 or ERp5-AGHA (background; white). Bound ERp5 or ERp5-AGHA was detected with anti-ERp5 antibody. ERp5 binding to αIIbβ3 vs GPIba, ERp5-AGHA binding to αIIbβ3 vs GPIbα, ERp5 binding to αIIbβ3 vs background, and ERp5-AGHA binding to αIIbβ3 vs background, **P < .005. Binding of ERp5 or ERp5-AGHA to GPIbα vs background was not statistically significant. Results are the average of 3 experiments. Surface plasmon resonance was used to determine the binding constant for ERp5 with recombinant β3 integrin tagged with calmodulin in the presence (C) or absence of Mn++ (D). ERp5 was coated on the Biacore chip. Lines represent the fitted curves of ERp5 at concentrations of 0, 0.33, 0.66, 1.31, 2.63, 5.25, 10.25, 21, and 42 µM. The KD values for ERp5 interaction with the β3 subunit in the presence and absence of Mn++ were 21.7 μM and 19.1 μM, respectively. ERp5 did not bind to calmodulin alone. n.s., not significant; RU, relative units.

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