Tissue-specific expression of mKng1 and mKng2. (A) RT-PCR of mKng1- and mKng2-derived HK mRNA transcripts in murine tissues. PCR products were resolved using 0.9% agarose gel electropheresis, and stained using ethidium bromide. Arrows indicate the location of PCR products from mKng1- and mKng2-derived HK mRNA. The lane on the left side of the gel (M) contains a DNA ladder. GAPDH mRNA was amplified in parallel to control for the DNA content of individual samples. L indicates liver; Lu, lung; K, kidney; A, adrenal; Bl, bladder; Br, brain; Mu, muscle; Thy, thymus; Sp, spleen; and H, heart. (B) In vitro translation of the regions of liver- and kidney-derived cDNA encoding Val364 to Arg540 of mKng1 (and corresponding region of mKng2). cDNA was amplified using the primers depicted in Figure 3B. PCR products were cloned into pBluescript II KS+, and used to synthesize capped mRNAs. In vitro translation was performed in the presence of 35S-methionine, and labeled polypeptides detected using 15% SDS-PAGE and autoradiography. As demonstrated in this figure, liver cDNA yielded a slightly larger polypeptide than that derived from kidney, consistent with expression of mKng1-derived HK mRNA in the former, and mKng2-derived HK mRNA in the latter.