Fig. 1.
Fig. 1. Detection of hFIX in rhesus plasma. / (A) Schematic representation of ELISA in which hFIX in rhesus plasma was captured by anti-hFIX Abs (capture Ab). The level of hFIX antigen was then determined with an HRP-conjugated goat anti-hFIX polyclonal secondary Ab. (B) A typical standard curve obtained with our ELISA showing a relatively linear range for detection of hFIX above 1% to 25% of normal levels. (C) Western blot analysis. Rhesus plasma was spiked with a known concentration of hFIX (0-3000 ng/mL). The vitamin K–dependent proteins were then precipitated by using barium citrate, and 5 μg precipitated protein was analyzed by a Western blotting procedure using rhesus immune serum (RQ1305) as the primary Ab. A band (∼70 kDa) in the expected position for FIX on reducing gels was detected only in rhesus plasma spiked with hFIX.

Detection of hFIX in rhesus plasma.

(A) Schematic representation of ELISA in which hFIX in rhesus plasma was captured by anti-hFIX Abs (capture Ab). The level of hFIX antigen was then determined with an HRP-conjugated goat anti-hFIX polyclonal secondary Ab. (B) A typical standard curve obtained with our ELISA showing a relatively linear range for detection of hFIX above 1% to 25% of normal levels. (C) Western blot analysis. Rhesus plasma was spiked with a known concentration of hFIX (0-3000 ng/mL). The vitamin K–dependent proteins were then precipitated by using barium citrate, and 5 μg precipitated protein was analyzed by a Western blotting procedure using rhesus immune serum (RQ1305) as the primary Ab. A band (∼70 kDa) in the expected position for FIX on reducing gels was detected only in rhesus plasma spiked with hFIX.

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