15542136

Source:http://linkedlifedata.com/resource/pubmed/id/15542136

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Predicate	Object
rdf:type	pubmed:Citation
lifeskim:mentions	umls-concept:C0033268, umls-concept:C0079679, umls-concept:C0086022, umls-concept:C0206037, umls-concept:C0442335, umls-concept:C0475208, umls-concept:C1705099
pubmed:issue	2
pubmed:dateCreated	2004-11-15
pubmed:abstractText	The goal of the present study was to develop an efficient transient transfection method for large-scale production of high titer lentivirus vector stocks of eight different pseudotypes. The envelope genes used for this purpose were those from VSV-G, Mokola, Rabies, MLV-Ampho, MLV-10A1, LCMV-WE, and LCMV-Arm53b. All envelopes were cloned into phCMV, which yielded lentivirus vector titers one, two, or three orders of magnitude higher than the original plasmids for the Rabies, MLV-10A1, and MLV-Ampho envelopes, respectively. When these newly constructed envelope expression plasmids were used for packaging, treatment with sodium butyrate resulted in almost five-fold increase in titers for some of the pseudotypes, had no effect for others (VSV-G and Rabies), and negatively impacted titers for the LCMV-derived pseudotypes. Production of vectors in serum-free media yielded titers only slightly lower than those obtained in the presence of serum. The efficiency of concentrating vector supernatants by ultracentrifugation or ultrafiltration was compared, with higher recovery efficiencies for the latter method, but the highest titers for most pseudotypes were obtained by ultracentrifugation. The best conditions for each individual pseudotype yielded lentivirus vector stocks with titers above 1 x 10(9) tu/mL for most pseudotypes, and higher than 1 x 10(10) tu/mL for VSV-G.
pubmed:language	eng
pubmed:journal	http://linkedlifedata.com/resource/pubmed/journal/8005839
pubmed:citationSubset	IM
pubmed:chemical	http://linkedlifedata.com/resource/pubmed/chemical/Viral Envelope Proteins, http://linkedlifedata.com/resource/pubmed/chemical/Viral Fusion Proteins
pubmed:status	MEDLINE
pubmed:month	Dec
pubmed:issn	0166-0934
pubmed:author	pubmed-author:CrombleholmeTimothyT, pubmed-author:FlakeAlan WAW, pubmed-author:Sena-EstevesMiguelM, pubmed-author:SteffensSabineS, pubmed-author:TebbetsJessica CJC
pubmed:issnType	Print
pubmed:day	15
pubmed:volume	122
pubmed:owner	NLM
pubmed:authorsComplete	Y
pubmed:pagination	131-9
pubmed:dateRevised	2007-11-15
pubmed:meshHeading	pubmed-meshheading:15542136-Cell Line, pubmed-meshheading:15542136-Ebolavirus, pubmed-meshheading:15542136-Genetic Vectors, pubmed-meshheading:15542136-HIV-1, pubmed-meshheading:15542136-Lentivirus, pubmed-meshheading:15542136-Lymphocytic choriomeningitis virus, pubmed-meshheading:15542136-Plasmids, pubmed-meshheading:15542136-Transduction, Genetic, pubmed-meshheading:15542136-Transfection, pubmed-meshheading:15542136-Vesicular stomatitis Indiana virus, pubmed-meshheading:15542136-Viral Envelope Proteins, pubmed-meshheading:15542136-Viral Fusion Proteins
pubmed:year	2004
pubmed:articleTitle	Optimized large-scale production of high titer lentivirus vector pseudotypes.
pubmed:affiliation	Department of Surgery, The Children's Hospital of Philadelphia, Abramson Research Center, 3615 Civic Center Blvd., Philadelphia, PA 19104, USA. msesteves@partners.org
pubmed:publicationType	Journal Article