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Last update 08 May 2025

GPR142

Last update 08 May 2025

Basic Info

Synonyms

G protein-coupled receptor 142, G-protein coupled receptor PGR2, GPR142

+ [2]

Introduction

Orphan receptor.

Drugs associated with GPR142

GPR142 agonists (Merck Research Laboratories)

Target

GPR142

Mechanism

GPR142 agonists

Active Org.

Merck Research Laboratories Massachusetts LLC

Originator Org.

Merck Research Laboratories Massachusetts LLC

Active Indication

Diabetes Mellitus, Type 2

Inactive Indication-

Drug Highest PhasePreclinical

First Approval Ctry. / Loc.-

First Approval Date20 Jan 1800

LY-3325656

Target

GPR142

Mechanism

GPR142 agonists

Active Org.-

Originator Org.

Eli Lilly & Co.

Active Indication-

Inactive Indication

Diabetes Mellitus, Type 2

Drug Highest PhasePending

First Approval Ctry. / Loc.-

First Approval Date20 Jan 1800

GPR142 agonists (Amgen)

Target

GPR142

Mechanism

GPR142 agonists

Active Org.-

Originator Org.

Amgen, Inc.

Active Indication-

Inactive Indication

Diabetes Mellitus, Type 2

Drug Highest PhasePending

First Approval Ctry. / Loc.-

First Approval Date20 Jan 1800

Clinical Trials associated with GPR142

NCT03115099

/ CompletedPhase 1

A Safety, Tolerability, Pharmacokinetic, and Pharmacodynamic Study of LY3325656 After Single Dose in Healthy Subjects and Patients With Type 2 Diabetes

The aim of this trial is to evaluate the safety of single doses of a study drug known as LY3325656 that is given orally to healthy participants and participants with type 2 diabetes. Information about any side effects that may occur will be collected.
It will also investigate how much of the study drug gets into the blood stream, and how long it takes the body to get rid of it.
The study consists of two parts. Part A will study healthy participants over approximately 12 weeks and Part B will study participants with type 2 diabetes over approximately 5 weeks, excluding screening. Screening is required within 28 days of the start of the study.

Start Date31 May 2017

Sponsor / Collaborator

Eli Lilly & Co.

100 Clinical Results associated with GPR142

100 Translational Medicine associated with GPR142

0 Patents (Medical) associated with GPR142

Literatures (Medical) associated with GPR142

18 Apr 2025·Beijing da xue xue bao. Yi xue ban = Journal of Peking University. Health sciences

[Effect of CMTM6 on PD-L1 in Helicobacter pylori infected gastric epithelial cells].

Article

Author: Ning, Jing ; Fu, Weiwei ; Fu, Wei ; Zhang, Jing ; Ding, Shigang

OBJECTIVETo explore the changes of CKLF-like MARVEL transmembrane domain-containing 6 (CMTM6) and programmed death-ligand 1 (PD-L1) expression in gastric mucosal epithelial cells after Helicobacter pylori infection and the regulation of CMTM6 on PD-L1, and to analyze the mRNA expression differences before and after CMTM6 gene knock-out in helicobacter pylori infected gastric epithelial cells by microarray analysis.METHODSThe standard Helicobacter pylori strain ATCC 26695 was co-cultured with human gastric epithelial cell GES-1 for 6, 24 and 48 hours, and the mRNA and protein levels of CMTM6 and PD-L1 were detected by real-time quantitative PCR and Western blot. Using CRISPR/Cas9 to construct CMTM6 gene knockout plasmid and knockout CMTM6 gene of GES-1 cells. Helicobacter pylori was co-cultured with CMTM6 gene knockout and wild type GES-1 cells for 48 hours to detect PD-L1 transcription and protein level changes, and CMTM6 gene knockout GES-1 cells were treated with the proteasome inhibitor MG-132 to detect the changes in PD-L1 protein levels. Agilent Human ceRNA Microarray 2019 was used to detect the differentially expressed genes in CMTM6 gene knockout and wild-type GES-1 cells co-cultured with Hp for 48 hours, and the signal pathway of differentially expressed genes enrichment was analyzed by Kyoto Encyclopedia of Genes and Genomes (KEGG) database.RESULTSThe mRNA and protein levels of CMTM6 and PD-L1 in GES-1 cells were significantly up-regulated after Helicobacter pylori infection, and CMTM6 mRNA was most significantly up-regulated 48 hours after infection. After CMTM6 gene knockout, the CD274 gene transcription level of Helicobacter pylori infected GES-1 cells did not change significantly, but PD-L1 protein level was significantly down-regulated, and the PD-L1 level increased after the application of proteasome inhibitor MG-132. After CMTM6 gene knockout, 67 genes had more than two times of differential expression. The transcription levels of TMEM68, FERMT3, GPR142, ATP6V1FNB, NOV, UBE2S and other genes were significantly down-regulated. The transcription levels of PCDHGA6, CAMKMT, PDIA2, NTRK3, SPOCK1 and other genes were significantly up-regulated. After CMTM6 gene knockout, ubiquitin-conjugating enzyme E2S (UBE2S) gene expression was significantly down-regulated, which might affect protein ubiquitination degradation. After CMTM6 gene knockout, adrenoceptor alpha 1B (ADRA1B), cholinergic receptor muscarinic 1 (M1), CHRM1, platelet activating factor receptor (PTAFR) gene expression was significantly up-regulated.CONCLUSIONHelicobacter pylori infection up-regulates the expression level of CMTM6 in gastric mucosa cells, and CMTM6 can stabilize PD-L1 and maintain the protein level of PD-L1. CMTM6 gene knockout may affect biological behaviors such as protein ubiquitination and cell surface receptor expression.

01 Jan 2025·Diabetologia

Molecular mechanisms underlying glucose-dependent insulinotropic polypeptide secretion in human duodenal organoids

Article

Author: Reimann, Frank ; Alcaino, Constanza ; Miedzybrodzka, Emily L ; Bany Bakar, Rula ; Santos-Hernández, Marta ; Guccio, Nunzio ; Kay, Richard G ; Smith, Christopher A ; Gribble, Fiona M ; Davison, Adam

AbstractAims/hypothesisGlucose-dependent insulinotropic polypeptide (GIP) is an incretin hormone secreted by enteroendocrine K cells in the proximal small intestine. This study aimed to explore the function of human K cells at the molecular and cellular levels.MethodsCRISPR-Cas9 homology-directed repair was used to insert transgenes encoding a yellow fluorescent protein (Venus) or an Epac-based cAMP sensor (Epac-S-H187) in the GIP locus in human duodenal-derived organoids. Fluorescently labelled K cells were purified by FACS for RNA-seq and peptidomic analysis. GIP reporter organoids were employed for GIP secretion assays, live-cell imaging of Ca2+ using Fura-2 and cAMP using Epac-S-H187, and basic electrophysiological characterisation. The G protein-coupled receptor genes GPR142 and CASR were knocked out to evaluate roles in amino acid sensing.ResultsRNA-seq of human duodenal K cells revealed enrichment of several G protein-coupled receptors involved in nutrient sensing, including FFAR1, GPBAR1, GPR119, CASR and GPR142. Glucose induced action potential firing and cytosolic Ca2+ elevation and caused a 1.8-fold increase in GIP secretion, which was inhibited by the sodium glucose co-transporter 1/2 (SGLT1/2) blocker sotagliflozin. Activation of the long-chain fatty acid receptor free fatty acid receptor 1 (FFAR1) induced a 2.7-fold increase in GIP secretion, while tryptophan and phenylalanine stimulated secretion by 2.8- and 2.1-fold, respectively. While CASR knockout blunted intracellular Ca2+ responses, a CASR/GPR142 double knockout was needed to reduce GIP secretory responses to aromatic amino acids.Conclusions/interpretationThe newly generated human organoid K cell model enables transcriptomic and functional characterisation of nutrient-sensing pathways involved in human GIP secretion. Both calcium-sensing receptor (CASR) and G protein-coupled receptor 142 (GPR142) contribute to protein-stimulated GIP secretion. This model will be further used to identify potential targets for modulation of native GIP secretion in diabetes and obesity.Graphical Abstract

01 Jul 2024·Acta Pharmacologica Sinica

GPCRs involved in metabolic diseases: pharmacotherapeutic development updates

Review

Author: Jin, Cheng ; Chen, Hui ; Zhou, Yuan ; Liu, Li-Li ; Xie, Li ; Wu, Jian

G protein-coupled receptors (GPCRs) are expressed in a variety of cell types and tissues, and activation of GPCRs is involved in enormous metabolic pathways, including nutrient synthesis, transportation, storage or insulin sensitivity, etc. This review intends to summarize the regulation of metabolic homeostasis and mechanisms by a series of GPCRs, such as GPR91, GPR55, GPR119, GPR109a, GPR142, GPR40, GPR41, GPR43 and GPR120. With deep understanding of GPCR's structure and signaling pathways, it is attempting to uncover the role of GPCRs in major metabolic diseases, including metabolic syndrome, diabetes, dyslipidemia and nonalcoholic steatohepatitis, for which the global prevalence has risen during last two decades. An extensive list of agonists and antagonists with their chemical structures in a nature of small molecular compounds for above-mentioned GPCRs is provided as pharmacologic candidates, and their preliminary data of preclinical studies are discussed. Moreover, their beneficial effects in correcting abnormalities of metabolic syndrome, diabetes and dyslipidemia are summarized when clinical trials have been undertaken. Thus, accumulating data suggest that these agonists or antagonists might become as new pharmacotherapeutic candidates for the treatment of metabolic diseases.

News (Medical) associated with GPR142

19 Nov 2015

·www.biospace.com

C4X Discovery Release: Appointment Of Dr Clive Dix As Executive Chairman And Departure Of Piers Morgan As CEO

19 November 2015 – C4X Discovery Holdings plc (“C4XD” or the “Company”), a leader in rational drug discovery and design, today announces the appointment of Dr Clive Dix as Executive Chairman. Until today Dr Dix has served as non-executive Chairman of C4XD’s Board of Directors. As Executive Chairman, Dr Dix will build upon the strong achievements C4XD has made to date in fulfilling its ambition to become one of the world’s leading hubs for the discovery of novel drugs against critical therapeutic targets. Recent achievements include advances in its Orexin-1, IL-17, GPR142 and NRF-2 programmes and the signing of a collaboration with the Structural Genomics Consortium at Oxford University (‘SGC’). Dr Dix is widely recognised as one of the leading figures in the UK biotechnology sector, combining track records as a serially successful entrepreneur and an experienced pharmaceutical R&D executive. Most recently, Dr Dix was CEO of Convergence Pharmaceuticals, which was sold to Biogen in January this year for $675m. Prior to that, Dr Dix enjoyed successful exits with PowderMed Limited, Auralis Limited and PowderJect Pharmaceuticals plc, where he held the roles of CEO, Chairman and Head of R&D, respectively. Before his move into biotechnology, Dr Dix was UK Research Director for GlaxoWellcome. He currently serves as Chairman of Touchlight Genetics Ltd and Calchan Ltd, and was Chairman of the UK BioIndustry Association (BIA) from 2008-2010. As Executive Chairman Dr Dix will assume day-to-day operational responsibilities for C4XD from Piers Morgan, who steps down as CEO today to pursue opportunities outside the company. These changes to the Board take place with immediate effect. Dr Clive Dix, Executive Chairman of C4XD, commented: “I am delighted to take up this executive role with C4XD. The Company has made excellent progress with the discovery of ground-breaking molecules in recent months, such as small molecules against IL-17 for inflammation and autoimmune diseases, and we are close to entering the clinic with our lead Orexin-1 programme for the treatment of addiction. Additional corporate developments such as the deal with the SGC at Oxford leave us well-placed to apply our technology to a range of unmet therapeutic needs. Now is the time to capitalise upon these developments and take C4XD to the next level as one of the world’s leading hubs for the discovery of exciting new drug candidates against critical therapeutic targets. I look forward to helping the Company to achieve this goal. On behalf of the Board of Directors, I would like to thank Piers Morgan for his contributions as CEO of C4XD and wish him luck as he pursues new opportunities.”

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GPR142

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