Bars represent mean and SEM from duplicate cultures in four indep

Bars represent mean and SEM from duplicate cultures in four independent experiments. ***P<0.001, ** P<0.01, * P<0.05 different from medium control, +++ P<0.001, ++ P<0.01, + P<0.05 different from L. jensenii WT. Expression of functional mCV-N expression and anti-HIV activity Protein Tyrosine Kinase inhibitor is preserved in epithelia-associated L. jensenii strains Filtered sterile supernatants from 24 h L. jensenii colonized vaginal and endocervical cells were assessed for mCV-N recovery with western blot analysis on an SDS-PAGE gel probed with anti-CV-N antibodies. All mCV-N expressing strains (lanes 2–4; Figure 8a, lanes 4–5; Figure 8b) produced full length mCV-N as compared to a mCV-N standard

(lane 1; Figure 8b). As expected, no background binding to mCV-N was detected in cell culture supernatants derived from the MALP-2 or medium controls (lanes 6–7; Figure 8a) or from either the WT (lane 1; Figure 8a, lane 2; Figure 8b) or β-glucuronidase producing strains (lane 5; Figure 8a, lane 6; Figure 8b). No protein loss to filtration was observed when 1 μg of mCV-N standard was

spiked in 1 ml of medium and probed with anti-mCV-N antibody in a western blot pre and post-filtration (Figure 8c). Figure 8 Epithelial colonized L. jensenii preserve potent anti-HIV properties. Western blot from 24 h sterile supernatants collected from L. jensenii-colonized vaginal (Vk2/E6E7) www.selleckchem.com/products/dinaciclib-sch727965.html and endocervical (End1E6E7) epithelial cells demonstrate consistent preservation of modified Cyanovirin-N (mCV-N) expression in mCV-N producing strains. (Figure 8a) mCV-N producing bioengineered strains (L. jensenii 1153–1666,

2666 and 3666) located in lanes #2, 3 and 4 are contrasted to L. jensenii 1153 WT in lane #1, the β-glucuronidase expressing strain L. jensenii 1153–1646 in lane #5, MALP-2 control in lane #6, and medium control in lane #7. (Figure 8b) A mCV-N standard in lane #1 is compared to the mCV-N producing L. jensenii strains: L. jensenii 1153–1666 and 3666 in lanes #4 and #5 in contrast to the green florescent protein expressing strain PLEKHB2 L. jensenii 1153-gfp in lane #6, MALP-2 in lane #3 and medium control in lane #2. (Figure 8c) No loss to filtration is observed in western blot analyses of mCV-N before and after spiking one ml of media with one μg mCV-N. (Figure 8d) gp120 binding activity in one representative mCV-N producing L. jensenii 1153–1666 strain detected by a gp120 binding assay in sterile supernatants collected from 24 h L. jensenii colonized vaginal (Vk2/E6E7) epithelial culture. Data are from one representing three independent experiments. Gp120 binding activity was measured in 24 h filtered sterile supernatants from L. jensenii colonized cervical and vaginal epithelial cells. Only the mCV-N producing strain resulted in gp120 binding activity compared to the WT and β-glucuronidase producing strains, MALP-2 or medium control (Figure 8d). Data were replicated in multiple experiments not shown here.

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