Figure 1.
Figure 1. Biochemical identification of natural and synthetic bovine SAA1(46-112). (A) MCF-2 was prepurified as described in the “Materials and methods” and supplemental Methods. Finally, cation exchange chromatography fractions containing bovine MCF-2 were purified to homogeneity by RP-HPLC. Proteins were eluted in an acetonitrile gradient (0% to 80%; dashed green line). The protein concentration was reflected by the absorbance at 214 nm (A214 nm; solid blue line). In all purification steps, column fractions were screened for chemotactic activity using the semiautomated MultiScreen chemotaxis assay (dilution: 1/100), in which THP-1 cells score reproducibly in a sensitive manner (solid red line with squares). (B) Sodium dodecyl sulfate–polyacrylamide gel electrophoresis under reducing conditions of the RP-HPLC fractions 35 to 53 (20 µL/lane). Proteins were visualized by silver staining. Relative molecular mass (Mr) markers are shown in the left and right lanes. The arrowhead indicates the 7- to 8-kDa protein, corresponding to MCF-2. (C) Mass spectrometric analysis of MCF-2, identified as natural SAA1(46-112). Two percent of the RP-HPLC column flow was deviated to an electrospray ion trap mass spectrometer. (D) Mass spectrometric analysis of synthetic SAA1(46-112). SAA1(46-112) was chemically synthesized using Fmoc chemistry and purified via RP-HPLC. (C-D) The averaged mass spectra, the number of charges for the detected ions, ion intensities, and corresponding mass to charge ratios (m/z) are shown. The inserts show the deconvoluted mass spectra with the Mr of the uncharged proteins calculated using the Bruker deconvolution software.

Biochemical identification of natural and synthetic bovine SAA1(46-112). (A) MCF-2 was prepurified as described in the “Materials and methods” and supplemental Methods. Finally, cation exchange chromatography fractions containing bovine MCF-2 were purified to homogeneity by RP-HPLC. Proteins were eluted in an acetonitrile gradient (0% to 80%; dashed green line). The protein concentration was reflected by the absorbance at 214 nm (A214 nm; solid blue line). In all purification steps, column fractions were screened for chemotactic activity using the semiautomated MultiScreen chemotaxis assay (dilution: 1/100), in which THP-1 cells score reproducibly in a sensitive manner (solid red line with squares). (B) Sodium dodecyl sulfate–polyacrylamide gel electrophoresis under reducing conditions of the RP-HPLC fractions 35 to 53 (20 µL/lane). Proteins were visualized by silver staining. Relative molecular mass (Mr) markers are shown in the left and right lanes. The arrowhead indicates the 7- to 8-kDa protein, corresponding to MCF-2. (C) Mass spectrometric analysis of MCF-2, identified as natural SAA1(46-112). Two percent of the RP-HPLC column flow was deviated to an electrospray ion trap mass spectrometer. (D) Mass spectrometric analysis of synthetic SAA1(46-112). SAA1(46-112) was chemically synthesized using Fmoc chemistry and purified via RP-HPLC. (C-D) The averaged mass spectra, the number of charges for the detected ions, ion intensities, and corresponding mass to charge ratios (m/z) are shown. The inserts show the deconvoluted mass spectra with the Mr of the uncharged proteins calculated using the Bruker deconvolution software.

Close Modal
This Feature Is Available To Subscribers Only

or Create an Account

Close Modal
Close Modal