Figure 3
Figure 3. Effect of IR injury on renal TF mRNA expression and functional activity. (A,C,D) TF mRNA was measured in extracts of kidney tissue from WT (n = 12), WT hirudin-treated (n = 7-9/time point), and PAR-1−/− mice (n = 12) at varying times (2, 5, and 24 hours) following renal IR injury or sham surgery (n = 6). (All values are expressed relative to 18S ribosomal RNA, and data are shown as mean ± SEM.) TF mRNA was increased at 2 hours after reperfusion and remained elevated for 24 hours (at all points **P < .001). TF mRNA was not increased in any sham-operated WT or PAR-1−/− animals (WT only shown). (B,D,F) TF functional activity (measured from extracts of kidney tissue using a 1-stage prothrombin assay) was increased in WT mice (n = 16) or PAR-1−/− mice (n = 16) at varying times (2, 5, and 24 hours) following renal IR injury compared with sham surgery (n = 6) (at 2 and 24 hours, **P < .005; at 5 hours, ***P < .05). Renal TF activity was very low from low-TF mice at all time points, and WT hirudin-treated mice had relatively reduced levels of TF activity (n = 7-9/group). IR injury resulted in no significant difference in TF expression between WT and PAR-1−/− mice. (All values are expressed in relative units compared with a standard curve of rabbit thromboplastin in which a 1 in 10 dilution of standard was designated 100 units.)

Effect of IR injury on renal TF mRNA expression and functional activity. (A,C,D) TF mRNA was measured in extracts of kidney tissue from WT (n = 12), WT hirudin-treated (n = 7-9/time point), and PAR-1−/− mice (n = 12) at varying times (2, 5, and 24 hours) following renal IR injury or sham surgery (n = 6). (All values are expressed relative to 18S ribosomal RNA, and data are shown as mean ± SEM.) TF mRNA was increased at 2 hours after reperfusion and remained elevated for 24 hours (at all points **P < .001). TF mRNA was not increased in any sham-operated WT or PAR-1−/− animals (WT only shown). (B,D,F) TF functional activity (measured from extracts of kidney tissue using a 1-stage prothrombin assay) was increased in WT mice (n = 16) or PAR-1−/− mice (n = 16) at varying times (2, 5, and 24 hours) following renal IR injury compared with sham surgery (n = 6) (at 2 and 24 hours, **P < .005; at 5 hours, ***P < .05). Renal TF activity was very low from low-TF mice at all time points, and WT hirudin-treated mice had relatively reduced levels of TF activity (n = 7-9/group). IR injury resulted in no significant difference in TF expression between WT and PAR-1−/− mice. (All values are expressed in relative units compared with a standard curve of rabbit thromboplastin in which a 1 in 10 dilution of standard was designated 100 units.)

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