%0 Journal Article %1 Lambris:1983wy %A Lambris, J D %A SCHEINER, O %A Schulz, T F %A ALSENZ, J %A Dierich, M P %D 1983 %J Journal of Immunological Methods %K imported %N 3 %P 277--283 %T Coupling of C3b to erythrocytes by disulfide bond formation: preparation of EC3b for hemolytic and complement receptor assays. %U http://eutils.ncbi.nlm.nih.gov/entrez/eutils/elink.fcgi?dbfrom=pubmed&id=6197481&retmode=ref&cmd=prlinks %V 65 %X We describe a new method of preparing C3-coated erythrocytes by coupling C3 to thiol-activated erythrocytes. The procedure involves three steps. Firstly, sheep erythrocytes were treated with N-succinimidyl 3-(2-pyridyldithio) propionate (SPDP) to introduce 3-(2-pyridyldithio) propionyl residues into membrane proteins. Secondly, C3 was cleaved with trypsin or CoVF, Bb enzyme to obtain C3b exposing the SH group (C3b-SH). Finally, the C3b-SH was coupled to the thiol-activated erythrocytes (TA-E) through thiol/disulfide exchange to form the TA-EC3b conjugate. E coated with C3d was prepared by treating TA-EC3b with KSCN inactivated serum and plasmin. Studying the rosette formation between TA-EC3b or TA-EC3d and cells expressing C3b (CR1) and C3d (CR2) receptors and the inhibition thereof with anti-CR1 and anti-CR2 antibodies as well as with C3-sheep E membrane protein complexes, we found that TA-EC3b and TA-EC3d bound exclusively to CR1 and CR2, respectively. In addition, TA-EC3b like EAC1423b bound factors B and H as tested by hemolytic and direct binding assays. The advantage of TA-EC3 for complement receptor and hemolytic assays are the simplicity of the preparation method and the general applicability of the TA-EC3.

@article{Lambris:1983wy, abstract = {We describe a new method of preparing C3-coated erythrocytes by coupling C3 to thiol-activated erythrocytes. The procedure involves three steps. Firstly, sheep erythrocytes were treated with N-succinimidyl 3-(2-pyridyldithio) propionate (SPDP) to introduce 3-(2-pyridyldithio) propionyl residues into membrane proteins. Secondly, C3 was cleaved with trypsin or CoVF, Bb enzyme to obtain C3b exposing the SH group (C3b-SH). Finally, the C3b-SH was coupled to the thiol-activated erythrocytes (TA-E) through thiol/disulfide exchange to form the TA-EC3b conjugate. E coated with C3d was prepared by treating TA-EC3b with KSCN inactivated serum and plasmin. Studying the rosette formation between TA-EC3b or TA-EC3d and cells expressing C3b (CR1) and C3d (CR2) receptors and the inhibition thereof with anti-CR1 and anti-CR2 antibodies as well as with C3-sheep E membrane protein complexes, we found that TA-EC3b and TA-EC3d bound exclusively to CR1 and CR2, respectively. In addition, TA-EC3b like EAC1423b bound factors B and H as tested by hemolytic and direct binding assays. The advantage of TA-EC3 for complement receptor and hemolytic assays are the simplicity of the preparation method and the general applicability of the TA-EC3.}, added-at = {2017-12-08T05:18:19.000+0100}, author = {Lambris, J D and SCHEINER, O and Schulz, T F and ALSENZ, J and Dierich, M P}, biburl = {https://www.bibsonomy.org/bibtex/2773c0513dbe069aacfc611cfd9c57637/lambris}, date-added = {2017-12-08T03:21:02GMT}, date-modified = {2017-12-08T04:17:04GMT}, interhash = {1de00d43efd36d2e2714ac3ad7216cf6}, intrahash = {773c0513dbe069aacfc611cfd9c57637}, journal = {Journal of Immunological Methods}, keywords = {imported}, language = {English}, month = dec, number = 3, pages = {277--283}, pmid = {6197481}, rating = {0}, timestamp = {2017-12-08T05:18:19.000+0100}, title = {{Coupling of C3b to erythrocytes by disulfide bond formation: preparation of EC3b for hemolytic and complement receptor assays.}}, uri = {\url{papers3://publication/uuid/10B484EF-9D05-4010-8EA4-0D7EE6946BC6}}, url = {http://eutils.ncbi.nlm.nih.gov/entrez/eutils/elink.fcgi?dbfrom=pubmed&id=6197481&retmode=ref&cmd=prlinks}, volume = 65, year = 1983 }