A novel tandem repeat cloning technique for creation of multiple short peptide repeats to differentiate closely related antigens.


Journal

Journal of immunological methods
ISSN: 1872-7905
Titre abrégé: J Immunol Methods
Pays: Netherlands
ID NLM: 1305440

Informations de publication

Date de publication:
06 2019
Historique:
received: 15 09 2018
revised: 11 12 2018
accepted: 16 01 2019
pubmed: 21 1 2019
medline: 28 4 2020
entrez: 21 1 2019
Statut: ppublish

Résumé

Antibody cross-reactivity is a problem often associated with closely related antigens. This study was aimed to develop a method enabling differentiation of closely related toxins based on antigen designing strategy. The method involves identification of disparate amino acids (AA) confined to target antigen in comparison with two or more closely related antigens, their assembly into a DNA oligomer and further cloning as six tandem repeats (TR) using restriction and ligation strategy into a desired vector and finally generation of antigen specific antibodies. The practical utility of this method was demonstrated by generating and testing the specificity of polyclonal antibodies against staphylococcal enterotoxin C (SEC). Cross-reactivity is a problem often associated with SEC in immunoassays due to its amino acid sequence identity with staphylococcal enterotoxin B (SEB) (40-60%). To circumvent the same, the above-mentioned strategy was applied. Unique AA of SEC (36 AA) in comparison to SEB were selected, reassembled and with deduced corresponding nucleotides, an oligomer of 117 bases was designed. Using primers with restriction overhangs, three constructs were created each with two repeats using a common restriction site. The resulting three constructs were sequentially cloned into alternating restriction sites of pRSET A vector in directional orientation, expressed in E. coli for rTR/SEC protein which was used to generate specific polyclonal antibodies against SEC. Specificity was compared with antibody raised against whole SEC recombinant protein using Western blot and dot blot assays. High specificity was achieved through the developed strategy signifying its possible application to address cross-reactivity problem associated with closely related antigens.

Identifiants

pubmed: 30660621
pii: S0022-1759(18)30343-0
doi: 10.1016/j.jim.2019.01.008
pii:
doi:

Substances chimiques

Antibodies, Bacterial 0
Antigens, Bacterial 0
Enterotoxins 0
Epitopes 0
Peptide Fragments 0
enterotoxin B, staphylococcal 39424-53-8
enterotoxin C, staphylococcal 39424-54-9

Types de publication

Comparative Study Journal Article Research Support, Non-U.S. Gov't

Langues

eng

Sous-ensembles de citation

IM

Pagination

11-17

Informations de copyright

Copyright © 2019. Published by Elsevier B.V.

Auteurs

Sowmya Nagaraj (S)

Microbiology Division, Defence Food Research Laboratory, Siddarthanagar, Mysore, Karnataka 570011, India.

Prakash Narayana Reddy (PN)

Department of Biotechnology, Vignan's Foundation for Science, Technology and Research (Deemed to be University), Vadlamudi, Guntur District, Andhra Pradesh 522 213, India.

Shylaja Ramlal (S)

Microbiology Division, Defence Food Research Laboratory, Siddarthanagar, Mysore, Karnataka 570011, India. Electronic address: shylajaramlal@gmail.com.

Soumya Paul (S)

Microbiology Division, Defence Food Research Laboratory, Siddarthanagar, Mysore, Karnataka 570011, India.

Bhavani Peddayelachagiri (B)

Microbiology Division, Defence Food Research Laboratory, Siddarthanagar, Mysore, Karnataka 570011, India.

D Manmohan Parida (DM)

Microbiology Division, Defence Food Research Laboratory, Siddarthanagar, Mysore, Karnataka 570011, India.

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Classifications MeSH