Abstract:Ricin is a potent glycoprotein toxin that is structurally composed of two subunits joined via a disulfide bond: a ~30 kDa subunit A (RTA) and a ~32 kDa subunit B (RTB). There are fears of ricin being used as a weapon for warfare and terrorism and, as such, there is an increasing need for the development of immunodiagnostic reagents targeted towards this toxin. This article describes the production and characterization of a panel of six ricinspecific monoclonal IgG antibodies (mAbs), previously selected based u… Show more
“…To accomplish this metric, we started with previously described high-affinity sdAbs specific for three distinct epitopes on ricin [26] , [27] , and implemented a multi-step process for obtaining binders with improved melting temperature and solubility. Ricin is a potent toxin listed as a select agent by the CDC, and the ability to detect ricin remains a high priority [28] , [29] , [30] , [31] . The potential offered by these thermal stabilized sdAb reagents to eliminate the cold-chain makes them a highly attractive alternative to conventional monoclonal antibody and scFv binding reagents.…”
“…To accomplish this metric, we started with previously described high-affinity sdAbs specific for three distinct epitopes on ricin [26] , [27] , and implemented a multi-step process for obtaining binders with improved melting temperature and solubility. Ricin is a potent toxin listed as a select agent by the CDC, and the ability to detect ricin remains a high priority [28] , [29] , [30] , [31] . The potential offered by these thermal stabilized sdAb reagents to eliminate the cold-chain makes them a highly attractive alternative to conventional monoclonal antibody and scFv binding reagents.…”
“…In the competitive assay, only one antibody was required, the anti-BAP antibody possessing highest binding affinity with BAP should be used for immunization to achieve a higher competitive inhibition ratio. 40,41 Compared with other anti-BAP antibodies, the ab17272 exhibited the minimum K D . Therefore, the anti-BAP mAb (ab17272) was selected for the FM-LFIA.…”
Section: Screening the Optimal Anti-bap Antibodymentioning
A convenient, reliable, highly sensitive, and competitive fluorescent microsphere-lateral flow immunochromatographic assay (FM-LFIA) was developed for the quantitative detection of BAP for the first time.
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