![Establishing the type 2N VWD mouse model using a CRISPR/Cas9 strategy. (A) A gRNA and asymmetric single-stranded oligodeoxynucleotide homology-directed repair template spanning the predicted Cas9 cleavage site were designed to introduce 3 single nucleotide changes into the mouse Vwf gene. The 2354G>a [G785E] mutation causes type 2N VWD. The other 2 changes are silent mutations, 2346G>a and 2358G>c, which eliminate the Cas9-requisite protospacer adjacent motif sequence and create a diagnostic Xho I site for genotyping, respectively. (B) Schematic diagram of genotyping by PCR and Xho I restriction enzyme digestion. (C) PCR detection of the 2354G>a variant mouse Vwf gene for genotyping. DNA was purified from peripheral blood leukocytes, and a 796-bp fragment was amplified from the mouse Vwf gene. PCR product was digested with Xho I and run on 1.25% gel. A single uncut fragment of 796 bp is observed for the wild-type mouse Vwf PCR product because it does not contain an Xho I restriction enzyme site. Two fragments (585 and 211 bp) result from the mutated type 2N mouse Vwf gene after Xho I digestion. Thus, a VWF+/+ genotype results in a single 796-bp band, VWF2N/2N genotype is indicated by 585- and 211-bp bands, and VWF2N/+ mice exhibited 796-, 585-, and 211-bp bands.](https://ash.silverchair-cdn.com/ash/content_public/journal/bloodadvances/6/9/10.1182_bloodadvances.2021006353/5/advancesadv2021006353f1.png?Expires=1720808987&Signature=jM5ukaV51nudn0iJWCSQPuy8uoH55RzAXp7O0gbB6dNyzz3e~b~vHBh2D99ODTPkuvSdkyNOdDDUQho6DK0zAN8QrE0NgI-bqpG-1FU8XOycZ-lrF5SH78a-V8zw0C~uTDbfOvB1P6qtyTyEUxE9EU8BUZIVDwYXfGkul6~9675LiWQ8ztogAGADt6y9YAxSDavzFbfSNv8pUhuCs29JXXMijk4PPeKMTmnElvhUKdIThyDaKGLEkDvNfNGjG9mnng0LEAdmCLBKIaIc37KslPsrPbkGCsQ2Jewv1xP3onIvy-8cdQuGjmMvQnrrYywR-grVJw0afSty2Lvf7jjM5w__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
Establishing the type 2N VWD mouse model using a CRISPR/Cas9 strategy. (A) A gRNA and asymmetric single-stranded oligodeoxynucleotide homology-directed repair template spanning the predicted Cas9 cleavage site were designed to introduce 3 single nucleotide changes into the mouse Vwf gene. The 2354G>a [G785E] mutation causes type 2N VWD. The other 2 changes are silent mutations, 2346G>a and 2358G>c, which eliminate the Cas9-requisite protospacer adjacent motif sequence and create a diagnostic Xho I site for genotyping, respectively. (B) Schematic diagram of genotyping by PCR and Xho I restriction enzyme digestion. (C) PCR detection of the 2354G>a variant mouse Vwf gene for genotyping. DNA was purified from peripheral blood leukocytes, and a 796-bp fragment was amplified from the mouse Vwf gene. PCR product was digested with Xho I and run on 1.25% gel. A single uncut fragment of 796 bp is observed for the wild-type mouse Vwf PCR product because it does not contain an Xho I restriction enzyme site. Two fragments (585 and 211 bp) result from the mutated type 2N mouse Vwf gene after Xho I digestion. Thus, a VWF+/+ genotype results in a single 796-bp band, VWF2N/2N genotype is indicated by 585- and 211-bp bands, and VWF2N/+ mice exhibited 796-, 585-, and 211-bp bands.