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Full length Clone DNA of Human cullin 1
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CRISPR/Cas9 KO Plasmids consists of CUL-1-specific 20 nt guide RNA sequences derived from the GeCKO (v2) library. For CRISPR gene knockout, gRNA sequences direct the Cas9 protein to induce a site-specific double strand break (DSB)
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Image Search Results
Journal: Development (Cambridge, England)
Article Title: Genome-wide analysis reveals that Smad3 and JMJD3 HDM co-activate the neural developmental program.
doi: 10.1242/dev.078345
Figure Lengend Snippet: Fig. 1. Endogenous Smad3 and JMJD3 interact in NSCs. (A)Size-exclusion chromatography of NSC lysate showing co-elution of Smad3P and JMJD3, and the presence of Smad3 in the lower weight fractions. (B)Co-IP of mouse NSCs lysate using anti-Smad3P antibody or unrelated IgGs in the presence or absence of TGFfor 30 minutes. (C)Upper panel shows schematic representation of GST-Smad3 fragments: full length (FL), MH1 (1-155 aa), MH2 (199-425 aa) and linker domains that also contains MH2 (146-425 aa). Pull-down assay using GST-Smad3 fusion proteins and 293t cell extracts overexpressing Myc-JMJD3. Ponceau staining of GST-Smad3 proteins (lower panel). (D)Immunoblot from control knockdown (C KD) and JMJD3 knockdown (JMJD3 KD) cell extracts using the indicated antibodies. (E)Immunoblot showing Nestin expression prior to and after TGFtreatment for the indicated times in C KD and JMJD3 KD cells. Nestin levels (relative to Actin) were quantified by using the Image J software (graph on the right). Input (In) corresponds to 1% of the protein present in the whole-cell extract.
Article Snippet:
Techniques: Size-exclusion Chromatography, Co-Elution Assay, Co-Immunoprecipitation Assay, Pull Down Assay, Staining, Western Blot, Control, Knockdown, Expressing, Software