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Env was 6-fold reduced in the absence of Rev indicating that Rev is important for the production of infectious particles with VHenv. As expected, Rev did not influence the titer of VHnef lacking the RRE. An alternative explanation for the gfp expression observed could be pseudotransduction of GFP protein or mRNA. This is unlikely because GFP fluorescence 25033180 mediated by this phenomenon peaks at approximately 12 hours after infection and is hardly detectable after 48 hours [19?1]. Whether the detected titer reflects gfp expression from integrated or unintegrated lentiviral vector DNA is unknown. Thus, VHenv and VHnef encoded transcripts could be packaged, reverse transcribed and transferred to target cells, although the vector titers were approximately 25 to 65-fold lower than those obtained for VHgenomic.Encapsidation efficienciesIn order to analyze the influence of Rev on encapsidation of different lentiviral vector RNAs we extracted cytoplasmic and virion-associated RNA after cotransfection of HEK293T cells with the lentiviral vectors, expression plasmids for tat, VSV-G and gag/ gagpol with or without a rev expression plasmid. The purity of the cytoplasmic fraction obtained with the mild lysis method used was rigorously tested previously [12,13]. Virions from cell culture supernatants were Autophagy purified through a 30 sucrose cushion. Cytoplasmic and particle RNA fractions were digested with DNase to remove remaining transfected plasmid DNA. Quantification of all RNA species was possible by specific quantitative RT-PCR protocols (see Materials and Methods S1, adapted from [9]). These PCRs do not detect the sequences of the transcomplementing gag/gagpol, tat and rev expression plasmids with relevant efficiency (see Materials and Methods S1). Control reactions without RT revealed efficient removal of the transfected plasmid DNA (data not shown). For all vector RNA species Rev had no statistically significant effect on cytoplasmic RNA levels (figure 3A). This is consistent with previous observations by us and others demonstrating that in the absence of Rev high amounts of unspliced lentiviral vector RNA are present in the cytoplasm of transfected cells and that adding Rev increased cytoplasmic vector RNA levels only minimally [13,22?5]. This is unlikely due to large nuclear contamination of our cytoplasmic fraction, since the fractionation protocol was validated repeatedly in our previous publications [12,13]. Nuclear proteins could not be detected in the cytoplasmic fraction by Western blotting and contamination of the cytoplasmic fraction with the nuclear pre-glyceraldehyde 3-phosphate dehydrogenase (pre-GAPDH) mRNA ranges from only 3 to 7 of the total amount of pre-GAPDH mRNA in the cell [12,13]. Furthermore, the results obtained for the unspliced RNA ofDetermination of vector titersInfectious particles were produced by transient cotransfection of HEK293T cells with the lentiviral vector VHgenomic or VHenv or VHnef together with expression plasmids for tat, vesicular stomatitis virus G protein (VSV-G) and gag/gagpol in the absence or presence of a rev expression plasmid. Constant and high Gag/ GagPol levels were provided by the Autophagy codon-optimized and therefore Rev-independent gag/gagpol expression plasmid Hgpsyn. Similar amounts of Gag/GagPol are produced after cotransfection of Hgpsyn with or without a rev expression plasmid (figure 2A and [12,13,18]). Furthermore, Gag/GagPol levels were comparable to those detected after transfection of the cor.Env was 6-fold reduced in the absence of Rev indicating that Rev is important for the production of infectious particles with VHenv. As expected, Rev did not influence the titer of VHnef lacking the RRE. An alternative explanation for the gfp expression observed could be pseudotransduction of GFP protein or mRNA. This is unlikely because GFP fluorescence 25033180 mediated by this phenomenon peaks at approximately 12 hours after infection and is hardly detectable after 48 hours [19?1]. Whether the detected titer reflects gfp expression from integrated or unintegrated lentiviral vector DNA is unknown. Thus, VHenv and VHnef encoded transcripts could be packaged, reverse transcribed and transferred to target cells, although the vector titers were approximately 25 to 65-fold lower than those obtained for VHgenomic.Encapsidation efficienciesIn order to analyze the influence of Rev on encapsidation of different lentiviral vector RNAs we extracted cytoplasmic and virion-associated RNA after cotransfection of HEK293T cells with the lentiviral vectors, expression plasmids for tat, VSV-G and gag/ gagpol with or without a rev expression plasmid. The purity of the cytoplasmic fraction obtained with the mild lysis method used was rigorously tested previously [12,13]. Virions from cell culture supernatants were purified through a 30 sucrose cushion. Cytoplasmic and particle RNA fractions were digested with DNase to remove remaining transfected plasmid DNA. Quantification of all RNA species was possible by specific quantitative RT-PCR protocols (see Materials and Methods S1, adapted from [9]). These PCRs do not detect the sequences of the transcomplementing gag/gagpol, tat and rev expression plasmids with relevant efficiency (see Materials and Methods S1). Control reactions without RT revealed efficient removal of the transfected plasmid DNA (data not shown). For all vector RNA species Rev had no statistically significant effect on cytoplasmic RNA levels (figure 3A). This is consistent with previous observations by us and others demonstrating that in the absence of Rev high amounts of unspliced lentiviral vector RNA are present in the cytoplasm of transfected cells and that adding Rev increased cytoplasmic vector RNA levels only minimally [13,22?5]. This is unlikely due to large nuclear contamination of our cytoplasmic fraction, since the fractionation protocol was validated repeatedly in our previous publications [12,13]. Nuclear proteins could not be detected in the cytoplasmic fraction by Western blotting and contamination of the cytoplasmic fraction with the nuclear pre-glyceraldehyde 3-phosphate dehydrogenase (pre-GAPDH) mRNA ranges from only 3 to 7 of the total amount of pre-GAPDH mRNA in the cell [12,13]. Furthermore, the results obtained for the unspliced RNA ofDetermination of vector titersInfectious particles were produced by transient cotransfection of HEK293T cells with the lentiviral vector VHgenomic or VHenv or VHnef together with expression plasmids for tat, vesicular stomatitis virus G protein (VSV-G) and gag/gagpol in the absence or presence of a rev expression plasmid. Constant and high Gag/ GagPol levels were provided by the codon-optimized and therefore Rev-independent gag/gagpol expression plasmid Hgpsyn. Similar amounts of Gag/GagPol are produced after cotransfection of Hgpsyn with or without a rev expression plasmid (figure 2A and [12,13,18]). Furthermore, Gag/GagPol levels were comparable to those detected after transfection of the cor.

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Author: nucleoside analogue