# Chip phosphorylation stimulates the degradation of mutant transthyretin to attenuate cardiac amyloidosis

> **NIH NIH R01** · JOHNS HOPKINS UNIVERSITY · 2024 · $701,186

## Abstract

PROJECT SUMMARY/ABSTRACT
Cardiac amyloidosis can be caused by a mutation in transthyretin (TTR) (e.g. valine 122 to isoleucine, VI) [ATTR-
CM] that will aggregate when taken up by the myocardium, resulting in cytotoxicity and ultimately dysfunction.
The mechanisms underlying the pathogenesis of ATTR-CM remain unknown. Further, methods to enhance the
degradation of dissociated and deposited transthyretin is a critical unmet need. We reported protein kinase G
(PKG) can enhance protein degradation via the proteasome and lysosome to attenuate cardiac disease. We
recently uncovered that PKG also phosphorylates a ubiquitin ligase/co-chaperone, Chip (carboxyl terminus of
Hsc70-interacting protein), at serine 19 (human; S20, mouse). Chip is a primary mediator of cardiomyocyte
proteostasis by ubiquitinating and shuttling proteins for degradation. With new and exciting pilot data we show
PKG activity and Chip S19 phosphorylation (pS19) are uniquely depressed in ATTR-CM patients. We also reveal
cardiomyocytes isolated from ATTR-CM patients have reduced myofibrillar function. The field has been stymied
by lack of models, especially in vivo, and access to human tissue. We addressed these limitations by creating
novel models and a biorepository of biopsies from ATTR-CM patients. In vitro, we developed engineered heart
tissue (EHT) and cardiac organoids formed from human iPSC-derived cardiomyocytes and fibroblasts. To create
ATTR-CM in vitro we incubate EHTs in TTRVI (5 µM, same as ATTR-CM plasma) or culture cardiac organoids
with TTRVI hepatic organoids (excretes TTRVI at a similar concentration) in an interconnected microphysiological
device for 14 days, resulting in cellular uptake, protein aggregation, lower PKG activity, cell death, and (in EHTs)
reduced function. Our new TTRVI knock in mouse develops diastolic dysfunction, increased expression of fibrotic
genes, and decreased PKG signaling. Males and ovariectomized female mice, but not intact females, develop
ATTR-CM, similar to human ATTR-CM which affects men and post-menopausal women. Our pilot data shows
activating PKG or expressing a Chip pS19-mimic (ChipSE) facilitates the clearance of TTRVI to enhance cardiac
function (mice and EHTs) and reduce cytotoxicity (organoids). This project will provide new mechanistic insight
into ATTR-CM by testing the impact of PKG activity and Chip pS19 in vitro and in vivo, tests a new therapeutic
strategy, and determines the translational relevance in human patients. Aim 1 tests if PKG stimulation or ChipSE
attenuates markers of ATTR-CM in vitro and the degradative process (proteasome or lysosome) utilized to
remove TTR. We also developed and will further test a novel tool (PROTAC) specifically targeting Chip for TTR
to enhance TTRVI removal. In Aim 2, we test the ability of various PKG activators protect against ATTR-CM and
if this occurs in a Chip pS20 dependent manner. In Aim 3, we will test the relevance of PKG signaling and Chip
pS19 in human ATTR-CM. We further ...

## Key facts

- **NIH application ID:** 10882087
- **Project number:** 1R01HL169273-01A1
- **Recipient organization:** JOHNS HOPKINS UNIVERSITY
- **Principal Investigator:** Mark John Ranek
- **Activity code:** R01 (R01, R21, SBIR, etc.)
- **Funding institute:** NIH
- **Fiscal year:** 2024
- **Award amount:** $701,186
- **Award type:** 1
- **Project period:** 2024-09-01 → 2028-07-31

## Primary source

NIH RePORTER: https://reporter.nih.gov/project-details/10882087

## Citation

> US National Institutes of Health, RePORTER application 10882087, Chip phosphorylation stimulates the degradation of mutant transthyretin to attenuate cardiac amyloidosis (1R01HL169273-01A1). Retrieved via AI Analytics 2026-05-25 from https://api.ai-analytics.org/grant/nih/10882087. Licensed CC0.

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