Exon II of glucokinase (Gk) was deleted to produce a systemic
heterozygous Gk knockout (Gk+/−) mouse. The
relative expression levels of Gk in the heart, lung, liver, stomach, and
pancreas in Gk+/− mice ranged from 0.41–0.68 versus that in
wild (Gk+/+) mice. On the other hand, its expression levels in
the brain, adipose tissue, and muscle ranged from 0.95–1.03, and its expression levels in
the spleen and kidney were nearly zero. Gk knockout caused no remarkable
off-target effect on the expression of 7 diabetes causing genes (Shp,
Hnf1a, Hnf1b, Irs1,
Irs2, Kir6.2, and Pdx1) in 10 organs.
The glucose tolerance test was conducted to determine the blood glucose concentrations
just after fasting for 24 h (FBG) and at 2 h after high-glucose application (GTT2h). The
FBG-GTT2h plots obtained with the wild strain fed the control diet (CD),
Gk+/− strain fed the CD, and
Gk+/− strain fed the HFD were distributed in separate areas
in the FBG-GTT2h diagram. The respective areas could be defined as the normal state,
prediabetes state, and diabetes state, respectively. Based on the results, the criteria
for prediabetes could be defined for the Gk+/− strain
developed in this study.
In order to produce insulin-secreting cells with a high value of glucose-stimulated insulin secretion (GSIS) from mouse embryonic stem cells, we have developed an optimized 5-stage protocol by referring to culture conditions so far reported elsewhere. This protocol is characterized by 4 points: (1) use of an activin-free medium in the first stage, (2) use of gelatin/fibronectin coated culture dishes in 1-4 stages throughout, (3) removal of undifferentiated cells by cell sorter at the end of 4th stage, and (4) sedimental culture in the 5th stage. GSIS value of the produced cells reached 2.4, that was at a higher rank of those so far reported. The produced cells were transplanted in diabetes model mice but no remedy effect was observed. Then transplantation was conducted in pre-diabetes model mice, in which GSIS was impaired without affecting insulin producing function. The transplantation of 5 9 10 6 cells resulted in a marked improvement of glucose tolerance within 20 days. This effect decreased but was still observed at 120 days post-transplantation. This demonstrates the feasibility of the novel optimized protocol.
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