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. 2007 Nov 13;111(3):1274–1281. doi: 10.1182/blood-2007-06-092338

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© 2008 by The American Society of Hematology

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Construction of an mKng1-targeting vector. Gene disruption was accomplished using recombineering, with details concerning the construction of the mKng1-targeting vector provided in “Methods.” Briefly, the strategy used a 9-kb genomic fragment of BAC452G1 to construct a targeting vector with which an mKng1 knockout allele was created. In this allele, exon 10 of mKng1 was replaced by a PGKNeo cassette (exon 10 contains the splicing site for HK and LK; thus, disruption of this exon should prevent transcription of HK and LK mRNA).