Fig. 1.
Fig. 1. Detection of CXCR4 transcripts by RNase protection assay. mRNA was extracted from peripheral blood mononuclear cells, PHA-activated mononuclear cells, CD41+ cells, and platelets. tRNA served as a negative control. Samples of mRNA were hybridized with a specific CXCR4 riboprobe and a specific actin riboprobe, then digested with RNase T1. Protected fragments were analyzed on denaturing acrylamide gels. Sizes of the fragments were determined using labeled Msp I–digested pBR322.

Detection of CXCR4 transcripts by RNase protection assay. mRNA was extracted from peripheral blood mononuclear cells, PHA-activated mononuclear cells, CD41+ cells, and platelets. tRNA served as a negative control. Samples of mRNA were hybridized with a specific CXCR4 riboprobe and a specific actin riboprobe, then digested with RNase T1. Protected fragments were analyzed on denaturing acrylamide gels. Sizes of the fragments were determined using labeled Msp I–digested pBR322.

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