TY - JOUR
T1 - Octadecyl silica
T2 - A solid phase for protein purification by immunoadsorption
AU - Chiong, Mario
AU - Lavandero, Sergio
AU - Ramos, Rodrigo
AU - Aguillón, Juan Carlos
AU - Ferreira, Arturo
N1 - Funding Information:
i This work supported by Grants 88198 UNDP/WORLD BANK/ WHO Special Programme for Research and Training in Tropical Diseases; 191188 FONDECYT CHILE; M2901-8813 DTI, Universidad de Chile; Swedish Agency for Research and Cooperation (SAREC). S.L. and J.C.A. are fellows of Fundacion Andes-Chile and CONICYT-Chile, respectively. Correspondence should be addressed to M. Chiong, Casilla 233, Santiago 1, Chile.
PY - 1991/8/15
Y1 - 1991/8/15
N2 - Immunoaffinity chromatography involves binding of an antigen or antibody to a solid matrix, usually agarose, frequently using the cyanogen bromide method. These methods are laborious, rather expensive, and their use has been mostly restricted to immunopurifications on the microscale. We propose here the use of octadecyl silica (SiCl8) beads, a matrix for HPLC, as an alternative solid phase for protein immunopurification and immunoadsorption. Antibodies or antigens are strongly bound to SiCl8 by a simple incubation; radiolabeled antibodies can only be eluted from SiCl8 by detergent-containing solutions. After the remaining free binding sites have been saturated with bovine serum albumin, SiCl8 is incubated with the antigen- or antibody-containing crude preparations and is then poured into a minicolumn. The nonspecifically bound proteins are removed by washing; specific proteins are eluted by disruption of the antigen-antibody complexes with a low pH buffer. With this methodology, we have obtained high purity preparations of proteins in single steps, even when these proteins are present in trace amounts (picograms) in a complex mixture such as human serum. Similarly, specific antibodies against an intracellular parasite (Trypanosoma cruzi) were completely absorbed from human serum with SiCl8 coated with parasite antigens.
AB - Immunoaffinity chromatography involves binding of an antigen or antibody to a solid matrix, usually agarose, frequently using the cyanogen bromide method. These methods are laborious, rather expensive, and their use has been mostly restricted to immunopurifications on the microscale. We propose here the use of octadecyl silica (SiCl8) beads, a matrix for HPLC, as an alternative solid phase for protein immunopurification and immunoadsorption. Antibodies or antigens are strongly bound to SiCl8 by a simple incubation; radiolabeled antibodies can only be eluted from SiCl8 by detergent-containing solutions. After the remaining free binding sites have been saturated with bovine serum albumin, SiCl8 is incubated with the antigen- or antibody-containing crude preparations and is then poured into a minicolumn. The nonspecifically bound proteins are removed by washing; specific proteins are eluted by disruption of the antigen-antibody complexes with a low pH buffer. With this methodology, we have obtained high purity preparations of proteins in single steps, even when these proteins are present in trace amounts (picograms) in a complex mixture such as human serum. Similarly, specific antibodies against an intracellular parasite (Trypanosoma cruzi) were completely absorbed from human serum with SiCl8 coated with parasite antigens.
UR - http://www.scopus.com/inward/record.url?scp=0025910201&partnerID=8YFLogxK
UR - http://www.scopus.com/inward/citedby.url?scp=0025910201&partnerID=8YFLogxK
U2 - 10.1016/0003-2697(91)90353-U
DO - 10.1016/0003-2697(91)90353-U
M3 - Article
C2 - 1659249
AN - SCOPUS:0025910201
SN - 0003-2697
VL - 197
SP - 47
EP - 51
JO - Analytical Biochemistry
JF - Analytical Biochemistry
IS - 1
ER -