LONP1 targets HMGCS2 to protect mitochondrial function and attenuate chronic kidney disease

A

Fibrosis deposition of kidney tissues was determined by Sirius red staining in UUO model. Scale bar: 50 μm.

B

Quantification of fibrotic area in UUO model (n = 10 in each group, biological replicates).

C, D

Representative Western blot images and densitometric analysis of FN1, Collagen I, α‐SMA and Vimentin protein levels in kidney tissues of UUO model (n = 9–10 in each group, biological replicates).

E

qRT‐PCR analysis of FN1, Collagen III, α‐SMA, Vimentin and Periostin mRNA levels in kidney tissues of UUO different groups (n = 10 in each group, biological replicates).

F

Representative images of succinate dehydrogenase (SDH) staining in UUO model. Scale bar: 50 μm.

G, H

Fibrosis deposition of kidney tissues was determined by Sirius red staining and quantified in UIRI model (n = 10 in each group, biological replicates). Scale bar: 50 μm.

I, J

Western blot and densitometric analysis of FN1, Vimentin and Periostin protein levels in kidney tissues of UIRI model (n = 8–10 in each group, biological replicates).

K

qRT‐PCR analysis of FN1, Collagen I, Collagen III, α‐SMA and Vimentin mRNA levels in kidney tissues of UIRI different groups (n = 8–10 in each group, biological replicates).

Figure 8. Anti‐renal fibrosis and maintenance of mitochondrial function of LONP1 activator in UUO and UIRI models.