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Overexpression and purification of human immunodeficiency virus type 1 env derived epitopes in Escherichia coli

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dc.contributor.authorMi Jin Sohn-
dc.contributor.authorMi-Eun Lee-
dc.contributor.authorHyo-Soon Park-
dc.contributor.authorSang-Uk Nham-
dc.contributor.authorYoung Ik Lee-
dc.date.accessioned2017-04-19T08:45:14Z-
dc.date.available2017-04-19T08:45:14Z-
dc.date.issued1996-
dc.identifier.issn0168-1656-
dc.identifier.urihttps://oak.kribb.re.kr/handle/201005/3678-
dc.description.abstractIn order to develop a reliable and inexpensive serodiagnostic method, a part of envelope gene of HIV-1, gp120' and gp41' (HIV-1 env a.a. 295-474 and a.a. 556-647) was cloned into a T7 expression vector (pET3d). The fusion protein (gp120'-gp41') was overexpressed in Escherichia coli, then purified to homogeneity by a simple gel filtration chromatography. Western blot analysis and enzyme-linked immunosorbent assay (ELISA) using the purified fusion protein showed a high sensitivity and a specificity for the detection of anti HIV-1 antibodies in testing human plasma. These results suggest that the expression scheme employing a direct expression vector and the rapid purification method are reliable and applicable for obtaining a large quantity of HIV-1 env protein for diagnoses of HIV-1 infections.-
dc.publisherElsevier-
dc.titleOverexpression and purification of human immunodeficiency virus type 1 env derived epitopes in Escherichia coli-
dc.title.alternativeOverexpression and purification of human immunodeficiency virus type 1 env derived epitopes in Escherichia coli-
dc.typeArticle-
dc.citation.titleJournal of Biotechnology-
dc.citation.number3-
dc.citation.endPage216-
dc.citation.startPage211-
dc.citation.volume45-
dc.contributor.affiliatedAuthorMi Jin Sohn-
dc.contributor.affiliatedAuthorYoung Ik Lee-
dc.contributor.alternativeName손미진-
dc.contributor.alternativeName이미은-
dc.contributor.alternativeName박효순-
dc.contributor.alternativeName남상욱-
dc.contributor.alternativeName이영익-
dc.identifier.bibliographicCitationJournal of Biotechnology, vol. 45, no. 3, pp. 211-216-
dc.identifier.doi10.1016/0168-1656(95)00169-7-
dc.subject.keyworddirect expression-
dc.subject.keywordELISA-
dc.subject.keywordenvelope-
dc.subject.keywordepitope-
dc.subject.keywordescherichia coli-
dc.subject.keywordfusion protein-
dc.subject.keywordgp120-
dc.subject.keywordgp41-
dc.subject.keywordHIV-1-
dc.subject.keywordT7 expression vector-
dc.subject.localdirect expression-
dc.subject.localELISA-
dc.subject.localELISA (enzyme-liked immunosorbent assay)-
dc.subject.localEnzyme-linked immunosorbent assay(ELISA)-
dc.subject.localenzyme-linked immunosorbent assay-
dc.subject.localenzyme-linked immunosorbent assay (ELISA)-
dc.subject.localenvelope-
dc.subject.localEpitope-
dc.subject.localepitope-
dc.subject.localE. Coli-
dc.subject.localE. coli-
dc.subject.localE.coli-
dc.subject.localEscherichia Coli-
dc.subject.localEscherichia coli-
dc.subject.localEscherichia coli.-
dc.subject.localescherichia coil-
dc.subject.localescherichia coli-
dc.subject.localFusion protein-
dc.subject.localfusion protein-
dc.subject.localgp120-
dc.subject.localgp41-
dc.subject.localgp41'-
dc.subject.localHIV-1-
dc.subject.localHIV1-
dc.subject.localT7 expression vector-
dc.description.journalClassY-
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