Novel method demonstrates differential ligand activation and phosphatase-mediated deactivation of insulin receptor tyrosine-specific phosphorylation

Anne M Cieniewicz; Philip R Cooper; Jennifer McGehee; Russell B Lingham; Anthony J Kihm

doi:10.1016/j.cellsig.2016.05.001

Novel method demonstrates differential ligand activation and phosphatase-mediated deactivation of insulin receptor tyrosine-specific phosphorylation

Cell Signal. 2016 Aug;28(8):1037-47. doi: 10.1016/j.cellsig.2016.05.001. Epub 2016 May 4.

Authors

Anne M Cieniewicz¹, Philip R Cooper², Jennifer McGehee², Russell B Lingham², Anthony J Kihm³

Affiliations

¹ Biologics Research, Janssen BioTherapeutics, Janssen R & D Spring House, PA 19477, USA. Electronic address: ACieniew@its.jnj.com.
² Biologics Research, Janssen BioTherapeutics, Janssen R & D Spring House, PA 19477, USA.
³ Biologics Research, Janssen BioTherapeutics, Janssen R & D Spring House, PA 19477, USA. Electronic address: AKihm@its.jnj.com.

PMID: 27155325
DOI: 10.1016/j.cellsig.2016.05.001

Abstract

Insulin receptor signaling is a complex cascade leading to a multitude of intracellular functional responses. Three natural ligands, insulin, IGF1 and IGF2, are each capable of binding with different affinities to the insulin receptor, and result in variable biological responses. However, it is likely these affinity differences alone cannot completely explain the myriad of diverse cellular outcomes. Ligand binding initiates activation of a signaling cascade resulting in phosphorylation of the IR itself and other intracellular proteins. The direct catalytic activity along with the temporally coordinated assembly of signaling proteins is critical for insulin receptor signaling. We hypothesized that determining differential phosphorylation among individual tyrosine sites activated by ligand binding or dephosphorylation by phosphatases could provide valuable insight into insulin receptor signaling. Here, we present a sensitive, novel immunoassay adapted from Meso Scale Discovery technology to quantitatively measure changes in site-specific phosphorylation levels on endogenous insulin receptors from HuH7 cells. We identified insulin receptor phosphorylation patterns generated upon differential ligand activation and phosphatase-mediated deactivation. The data demonstrate that insulin, IGF1 and IGF2 elicit different insulin receptor phosphorylation kinetics and potencies that translate to downstream signaling. Furthermore, we show that insulin receptor deactivation, regulated by tyrosine phosphatases, occurs distinctively across specific tyrosine residues. In summary, we present a novel, quantitative and high-throughput assay that has uncovered differential ligand activation and site-specific deactivation of the insulin receptor. These results may help elucidate some of the insulin signaling mechanisms, discriminate ligand activity and contribute to a better understanding of insulin receptor signaling. We propose this methodology as a powerful approach to characterize agonists and antagonists of the insulin receptor and can be adapted to serve as a platform to evaluate ligands of alternate receptor systems.

Keywords: IGF1; IGF2; Insulin receptor; Metabolic; Phosphorylation; Signaling.

MeSH terms

Cell Line, Tumor
Enzyme Activation / drug effects
Humans
Insulin / pharmacology
Insulin-Like Growth Factor I / pharmacology
Insulin-Like Growth Factor II / pharmacology
Kinetics
Ligands
Models, Biological
Phosphorylation / drug effects
Phosphoserine / metabolism*
Protein Tyrosine Phosphatases / metabolism*
Proto-Oncogene Proteins c-akt / metabolism
Receptor, Insulin / metabolism*
Time Factors
Vanadates / pharmacology

Substances

Insulin
Ligands
Phosphoserine
Vanadates
Insulin-Like Growth Factor I
Insulin-Like Growth Factor II
Receptor, Insulin
Proto-Oncogene Proteins c-akt
Protein Tyrosine Phosphatases