Uso de partículas magnéticas en la purificación de anticuerpos IgM contra Taenia solium
Perez, L. Agueda; Castillo Berrios, Yesenia; Espinoza Guerrero, Cindy; Toribio, Luz M.; Santos, Yesica; Martel, Kevin S.; Wilkins, P.P.; Bustos Palomino, Javier Arturo; García Lescano, Héctor Hugo; Castro-Sesquen, Y.E.; Gilman, Robert Hugh; Gonzalez Zariquiey, Armando Emiliano; Tsang, V.C.W.; Rodriguez, S.; Gonzalez, I.; Saavedra Pastor, Herbert; Sanchez, S.; Martinez, M.; Verastegui Pimentel, Manuela Renee; Zimic-Peralta, Mirko Juan; Santivañez, Saul; Mayta, Holger; Pajuelo Travezaño, Monica Jhenny; Arroyo Hurtado, Gianfranco; Lopez, M.T.; Gomez, L.; Vargas, A.; Gavidia, C.M.; Moyano, L.M.; Gamboa Morán, Ricardo; Muro Ecca, Claudio Alberto; Vichez, P.; O´neal, S.; Handali, S.; Noh, J.; Nash, T.E.; Mahanty, S.; Friedland, J.
Fecha:
2020
Resumen:
The use of L protein coupled magnetic particles for the concentration and purification of immunoglobulin M (mIgM) monoclonal antibodies against Taenia solium was evaluated. Three concentration methods and different elution times were evaluated and the ratio of particles to the ratio of mIgM was optimized. It is demonstrated that: 1) with the use of magnetic particles, a previous concentration of mIgM is not required, which reduces the manipulation of the antibodies and improves the recovery, 2) the use of a binding buffer can be omitted, since the pH of most cell culture supernatants are neutral, and 3) longer elution times (~ 45 minutes) are needed to increase recovery to a level greater than 80%. The study demonstrates that the use of L protein-coupled magnetic particles is a simple and efficient tool for mIgM concentration and purification.
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