Mapping the C1q Binding Site on Paramyosin

To identify and locate the complement C1q binding site on TsPmy, the full-length T. spiralis paramyosin (TsPmy1-885aa, NCBI accession numbers for nucleotides sequence: EF429310.1 and protein sequence: ABO09862.1) was expressed as recombinant protein using a baculovirus insect expression system (Invitrogen, Carlsbad, CA, USA), and the subsequent fragments of TsPmy, with 30 amino acids overlapped (TsPmy1-315aa, TsPmy286-600aa, TsPmy571-885aa), were sub-cloned and expressed in an E. coli expression system (Novagen, Merck, Darmstadt, Germany) as described in [4 (link)]. Further fragmenting expression on the C1q-binding fragments of TsPmy1-315aa (TsPmy1-125aa, 96-220aa, 191-315aa) and TsPmy191-315aa (TsPmy191-245aa, 226-280aa, 261-315aa) was performed in E. coli. All recombinant proteins were expressed with 6-histidine tag and purified by nickel affinity chromatograph (GE Healthcare, Boston, MA, USA).

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Wang Z., Hao C., Huang J., Zhuang Q., Zhan B, & Zhu X. (2018). Mapping of the complement C1q binding site on Trichinella spiralis paramyosin. Parasites & Vectors, 11, 666.

Publication 2018

baculovirus insect expression system nickel affinity chromatograph

Affinity chromatograph Amino acids Baculovirus Binding site Complement c1q E coli Histidine Insect Nickel Nucleotides Paramyosin Protein sequence Recombinant proteins

Corresponding Organization :

Other organizations : Capital Medical University, Baylor College of Medicine

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Variable analysis

independent variables

Expression of full-length TsPmy (TsPmy1-885aa) as recombinant protein using a baculovirus insect expression system
Expression of TsPmy fragments (TsPmy1-315aa, TsPmy286-600aa, TsPmy571-885aa) as recombinant proteins in an E. coli expression system
Further fragmentation and expression of TsPmy1-315aa (TsPmy1-125aa, 96-220aa, 191-315aa) and TsPmy191-315aa (TsPmy191-245aa, 226-280aa, 261-315aa) in E. coli

dependent variables

Identification and location of the complement C1q binding site on TsPmy

control variables

All recombinant proteins were expressed with 6-histidine tag
All recombinant proteins were purified by nickel affinity chromatography

controls

No positive or negative controls were explicitly mentioned in the input protocol.

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