Cold Storage Followed by Transplantation Induces Immunoproteasome in Rat Kidney Allografts: Inhibition of Immunoproteasome Does Not Improve Function

Dinesh Bhattarai; Seong-Ok Lee; Neelam Joshi; Se-Ran Jun; Sorena Lo; Li Jiang; Neriman Gokden; Nirmala Parajuli

doi:10.34067/KID.0000000000000368

Cold Storage Followed by Transplantation Induces Immunoproteasome in Rat Kidney Allografts: Inhibition of Immunoproteasome Does Not Improve Function

Kidney360. 2024 May 1;5(5):743-752. doi: 10.34067/KID.0000000000000368. Epub 2024 Feb 2.

Authors

Dinesh Bhattarai¹, Seong-Ok Lee¹, Neelam Joshi¹, Se-Ran Jun², Sorena Lo¹, Li Jiang¹, Neriman Gokden³, Nirmala Parajuli^{1

4}

Affiliations

¹ Department of Pharmacology and Toxicology, University of Arkansas for Medical Sciences, Little Rock, Arkansas.
² Department of Biomedical Informatics, University of Arkansas for Medical Sciences, Little Rock, Arkansas.
³ Department of Pathology, University of Arkansas for Medical Sciences, Little Rock, Arkansas.
⁴ Division of Nephrology, University of Arkansas for Medical Sciences, Little Rock, Arkansas.

Abstract

Key Points:

Cold storage (CS) increases the severity of graft dysfunction in a time-dependent manner, and prolonged CS decreases animal survival.
CS plus transplant increases iproeasome levels/assembly in renal allografts; IFN-γ is a potential inducer of the iproteasome.
Inhibiting iproteasome ex vivo during renal CS did not confer graft protection after transplantation.

Background: It is a major clinical challenge to ensure the long-term function of transplanted kidneys. Specifically, the injury associated with cold storage (CS) of kidneys compromises the long-term function of the grafts after transplantation. Therefore, the molecular mechanisms underlying CS-related kidney injury are attractive therapeutic targets to prevent injury and improve long-term graft function. Previously, we found that constitutive proteasome function was compromised in rat kidneys after CS followed by transplantation. Here, we evaluated the role of the immunoproteasome (iproteasome), a proteasome variant, during CS followed by transplantation.

Methods: Established in vivo rat kidney transplant model with or without CS containing vehicle or iproteasome inhibitor (ONX 0914) was used in this study. The iproteasome function was performed using rat kidney homogenates and fluorescent-based peptide substrate specific to β5i subunit. Western blotting and quantitative RT-PCR were used to assess the subunit expression/level of the iproteasome (β5i) subunit.

Results: We demonstrated a decrease in the abundance of the β5i subunit of the iproteasome in kidneys during CS, but β5i levels increased in kidneys after CS and transplant. Despite the increase in β5i levels and its peptidase activity within kidneys, inhibiting β5i during CS did not improve graft function after transplantation.

Summary: These results suggest that the pharmacologic inhibition of immunoproteasome function during CS does not improve graft function or outcome. In light of these findings, future studies targeting immunoproteasomes during both CS and transplantation may define the role of immunoproteasomes on short-term and long-term kidney transplant outcomes.

Publication types

Letter

MeSH terms

Allografts*
Animals
Kidney / immunology
Kidney / metabolism
Kidney Transplantation*
Male
Organ Preservation / methods
Proteasome Endopeptidase Complex* / metabolism
Proteasome Inhibitors / pharmacology
Rats

Substances

Proteasome Endopeptidase Complex
Proteasome Inhibitors

Abstract

Publication types

MeSH terms

Substances

Grants and funding