Figure 6
Figure 6. Functional recovery and gene expression. (A) Whole blood clotting assay. Blood was withdrawn from the eye in a capillary tube. The clotting time was determined by visual observation of the clot formation. The results showed a significant drop in the blood clotting time in HAT mice after 5 months of transplantation compared with the HA mice. The number of mice tested (n) in each condition is mentioned in the figure. *P < .01. (B) Tail-clip challenge. The numbers of surviving and dead mice are shown after tail clip. In HAT mice, 80% were protected from death resulting from blood loss. The numbers of mice tested in each group are as follows: WT (9 mice), HA (13 mice), HAT-2 months (13 mice), HAT-5 months (17 mice), and HAT-12 months (14 mice). (C) The rationale for designing primers to amplify a sequence of the FVIII A3 domain. It is difficult to reverse transcribe across the neo sequence resulting from the presence of high G + C content in HA mice. (D) The RT-PCR analysis for the synthesis of the target amplicon. HAT1-3 mice show the synthesis of a 637-bp amplicon, the same as in WT mice. The same gene product was absent in both the knockout mice (HA1 and HA2).

Functional recovery and gene expression. (A) Whole blood clotting assay. Blood was withdrawn from the eye in a capillary tube. The clotting time was determined by visual observation of the clot formation. The results showed a significant drop in the blood clotting time in HAT mice after 5 months of transplantation compared with the HA mice. The number of mice tested (n) in each condition is mentioned in the figure. *P < .01. (B) Tail-clip challenge. The numbers of surviving and dead mice are shown after tail clip. In HAT mice, 80% were protected from death resulting from blood loss. The numbers of mice tested in each group are as follows: WT (9 mice), HA (13 mice), HAT-2 months (13 mice), HAT-5 months (17 mice), and HAT-12 months (14 mice). (C) The rationale for designing primers to amplify a sequence of the FVIII A3 domain. It is difficult to reverse transcribe across the neo sequence resulting from the presence of high G + C content in HA mice. (D) The RT-PCR analysis for the synthesis of the target amplicon. HAT1-3 mice show the synthesis of a 637-bp amplicon, the same as in WT mice. The same gene product was absent in both the knockout mice (HA1 and HA2).

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