Ca²⁺ Influx Channel Inhibitor SARAF Protects Mice From Acute Pancreatitis.

BACKGROUND & AIMS:Pancreatitis is characterized by increased influx of Ca²⁺ into acinar cells, by unknown mechanisms. Inhibitors of Ca²⁺ influx channels could be effective in treating acute pancreatitis, but these have deleterious side effects that can result in death. We investigated the expression patterns and functions of acinar cell Ca²⁺ channels and factors that regulate them during development of acute pancreatitis, along with changes in the channel inactivator store-operated calcium entry-associated regulatory factor We investigated whether is a target for treatment of acute pancreatitis and its status in human with pancreatitis. METHODS:We generated mice that expressed duanyu1800F tagged with hemagglutinin, using CRISPR/Cas9 gene editing, and isolated acinar cells. We also performed studies with Saraf^-/- mice, Saraf^zf/zf mice, mice without disruption of Saraf (control mice), and mice that overexpress fluorescently labeled duanyu1800F in acinar cells. We analyzed interactions between stromal interaction molecule 1 (STIM1) and duanyu1800F in HEK cells stimulated with carbachol using fluorescence resonance energy transfer microscopy and immunoprecipitation. Mice were given injections of caerulein or L-arginine to induce pancreatitis. Pancreatic tissues and blood samples were collected and levels of serum amylase, trypsin, tissue damage, inflammatory mediators, and inflammatory cells were measured. We performed quantitative polymerase chain reaction analyses of pancreatic tissues from 6 organ donors without pancreatic disease (controls) and 8 patients with alcohol-associated pancreatitis. RESULTS:Pancreatic levels of Ca²⁺ influx channels or STIM1 did not differ significantly between acinar cells from mice with vs. without pancreatitis. By contrast, pancreatic levels of Saraf messenger RNA and duanyu1800F protein initially markedly increased but then decreased during cell stimulation or injection of mice with caerulein, resulting in excessive Ca²⁺ influx. STIM1 interacted stably with duanyu1800F following stimulation of HEK or mouse acinar cells with physiologic levels of carbachol, but only transiently following stimulation with pathologic levels of carbachol, leading to excessive Ca²⁺ influx. We observed reduced levels of duanyu1800F messenger RNA in pancreatic tissues from patients with pancreatitis, compared with controls. duanyu1800F knockout mice developed more severe pancreatitis than control mice after administration of caerulein or L-arginine, and pancreatic acinar cells from these mice had significant increases in Ca²⁺ influx. Conversely, overexpression of duanyu1800F in acini reduced Ca²⁺ influx, eliminated inflammation, and reduced severity of acute pancreatitis. CONCLUSIONS:In mice with pancreatitis, duanyu1800F initially increases but is then degraded, resulting in excessive, pathological Ca²⁺ influx by acinar cells. duanyu1800F knockout mice develop more severe pancreatitis than control mice, whereas mice that express duanyu1800F from a transgene in acinar cells develop less-severe pancreatitis. duanyu1800F therefore appears to prevent pancreatic damage during development of acute pancreatitis. Strategies to stabilize or restore duanyu1800F to acinar cells might be developed for treatment of pancreatitis.

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