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dc.contributor.authorMéndez Scolari, José Emilio
dc.contributor.authorFlorentín Pavía, Marcos Marcelo
dc.contributor.authorMujica, M. P.
dc.contributor.authorRojas, N.
dc.contributor.authorSotelo Torres, Pablo Hernán 
dc.contributor.otherUniversidad Nacional de Asunción - Facultad de Ciencias Químicases
dc.date.accessioned2022-04-27T23:38:00Z
dc.date.available2022-04-27T23:38:00Z
dc.date.issued2019-03
dc.identifier.urihttp://hdl.handle.net/20.500.14066/3732
dc.description.abstractFilamentous bacteriophages are widely used in phage display technology. The most common quantification method is lysis plaque formation test (PFT). This technique has several disadvantages, and only quantifies infective phages and is not effective when phagemids are used. We developed a qPCR method directed against the M13 replication origin, which detects between 3.3 9 103 and 3.3 9 108 viral genome copies with a linearity of R2 = 0.9998. Using this method we were able to observe a difference of approximately ten more phages than with the PFT. This difference was not due to the presence of a free genome, which suggests the presence of non-infective particles. Using a DNaseI treatment, we observed the presence of 30% to 40% of unpackaged genome in recombinant phage modified in PIII or PVIII. The qPCR method with a DNase I treatment is an efficient method to quantify the total amount of filamentous phages.es
dc.description.sponsorshipCONACYT – Consejo Nacional de Ciencia y Tecnologíaes
dc.language.isoenges
dc.subject.classification6 Producción y tecnología industriales
dc.subject.otherPHAGE QUANTITATIONes
dc.subject.otherPHAGE DISPLAYes
dc.subject.otherQPCRes
dc.subject.otherPHAGEMIDSes
dc.titleA qPCR targeted against the viral replication origin designed to quantify total amount of filamentous phages and phagemidses
dc.typeresearch articlees
dc.identifier.doihttps://doi.org/10.1007/s12088-019-00798-xes
dc.description.fundingtextPROCIENCIAes
dc.issue.number365es
dc.journal.titleIndian Journal of Microbiologyes
dc.page.initial369es
dc.relation.projectCONACYTPINV15-224es
dc.rights.accessRightsopen accesses
dc.rights.copyright© Association of Microbiologists of India 2019es
dc.subject.ocdeFARMACOLOGIAes
dc.volume.number59es


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