ABSTRACT
AIM: To compare the damage of light-emitting diodes (LEDs) with different color rendering indexes (CRIs) to the ocular surface and retina of rats. METHODS: Totally 20 Sprague-Dawley (SD) rats were randomly divided into four groups: the first group was normal control group without any intervention, other three groups were exposed by LEDs with low (LED-L), medium (LED-M), and high (LED-H) CRI respectively for 12h a day, continuously for 4wk. The changes in tear secretion (Schirmer I test, SIt), tear film break-up time (BUT), and corneal fluorescein sodium staining (CFS) scores were compared at different times (1d before experiment, 2 and 4wk after the experiment). The histopathological changes of rat lacrimal gland and retina were observed at 4wk, and the expressions of tumor necrosis factor-α (TNF-α) and interleukin-6 (IL-6) in lacrimal gland were detected by immunofluorescence method. RESULTS: With the increase of light exposed time, the CFS value of each light exposed group continued to increase, and the BUT and SIt scores continued to decrease, which were different from the control group, and the differences between the light exposed groups were statistically significant. Hematoxylin-eosin (HE) results showed that the lacrimal glands of each exposed group were seen varying degrees of acinar atrophy, vacuole distribution, increasing of eosinophil granules, etc.; the retina showed obvious reduction of photoreceptor cell layer and changes in retinal thickness; LED-L group has the most significant change in all tests. Immunofluorescence suggested that the positive expressions of TNF-α and IL-6 in the lacrimal glands of each exposed group were higher than those of the control group. CONCLUSION: LED exposure for 4wk can cause the pathological changes of lacrimal gland and retina of rats, and increase the expression of TNF-α and IL-6 in lacrimal gland, the degree of damage is negatively correlated with the CRI.
ABSTRACT
Arrestins recognize different receptor phosphorylation patterns and convert this information to selective arrestin functions to expand the functional diversity of the G protein-coupled receptor (GPCR) superfamilies. However, the principles governing arrestin-phospho-receptor interactions, as well as the contribution of each single phospho-interaction to selective arrestin structural and functional states, are undefined. Here, we determined the crystal structures of arrestin2 in complex with four different phosphopeptides derived from the vasopressin receptor-2 (V2R) C-tail. A comparison of these four crystal structures with previously solved Arrestin2 structures demonstrated that a single phospho-interaction change results in measurable conformational changes at remote sites in the complex. This conformational bias introduced by specific phosphorylation patterns was further inspected by FRET and 1H NMR spectrum analysis facilitated via genetic code expansion. Moreover, an interdependent phospho-binding mechanism of phospho-receptor-arrestin interactions between different phospho-interaction sites was unexpectedly revealed. Taken together, our results provide evidence showing that phospho-interaction changes at different arrestin sites can elicit changes in affinity and structural states at remote sites, which correlate with selective arrestin functions.
Subject(s)
Receptors, Vasopressin/metabolism , beta-Arrestin 1/metabolism , Crystallography, X-Ray , HEK293 Cells , Humans , Mutation , Nuclear Magnetic Resonance, Biomolecular , Phosphopeptides/chemistry , Phosphopeptides/metabolism , Phosphorylation , Protein Conformation, alpha-Helical , Protein Domains/genetics , Receptors, Vasopressin/chemistry , Receptors, Vasopressin/ultrastructure , Recombinant Proteins/isolation & purification , Recombinant Proteins/metabolism , Recombinant Proteins/ultrastructure , beta-Arrestin 1/genetics , beta-Arrestin 1/isolation & purification , beta-Arrestin 1/ultrastructureABSTRACT
Characterization of the dynamic conformational changes in membrane protein signaling complexes by nuclear magnetic resonance (NMR) spectroscopy remains challenging. Here we report the site-specific incorporation of 4-trimethylsilyl phenylalanine (TMSiPhe) into proteins, through genetic code expansion. Crystallographic analysis revealed structural changes that reshaped the TMSiPhe-specific amino-acyl tRNA synthetase active site to selectively accommodate the trimethylsilyl (TMSi) group. The unique up-field 1H-NMR chemical shift and the highly efficient incorporation of TMSiPhe enabled the characterization of multiple conformational states of a phospho-ß2 adrenergic receptor/ß-arrestin-1(ß-arr1) membrane protein signaling complex, using only 5 µM protein and 20 min of spectrum accumulation time. We further showed that extracellular ligands induced conformational changes located in the polar core or ERK interaction site of ß-arr1 via direct receptor transmembrane core interactions. These observations provided direct delineation and key mechanism insights that multiple receptor ligands were able to induce distinct functionally relevant conformational changes of arrestin.
Subject(s)
Arrestin/chemistry , Arrestin/genetics , Arrestin/metabolism , Ligands , Proton Magnetic Resonance Spectroscopy/methods , Binding Sites , Crystallography, X-Ray , Humans , Models, Molecular , Phenylalanine , Protein Binding , Protein Conformation , Receptors, Adrenergic, beta-2/metabolism , Signal Transduction , beta-Arrestin 1/chemistry , beta-Arrestin 1/genetics , beta-Arrestin 1/metabolismABSTRACT
Acute hormone secretion triggered by G protein-coupled receptor (GPCR) activation underlies many fundamental physiological processes. GPCR signalling is negatively regulated by ß-arrestins, adaptor molecules that also activate different intracellular signalling pathways. Here we reveal that TRV120027, a ß-arrestin-1-biased agonist of the angiotensin II receptor type 1 (AT1R), stimulates acute catecholamine secretion through coupling with the transient receptor potential cation channel subfamily C 3 (TRPC3). We show that TRV120027 promotes the recruitment of TRPC3 or phosphoinositide-specific phospholipase C (PLCγ) to the AT1R-ß-arrestin-1 signalling complex. Replacing the C-terminal region of ß-arrestin-1 with its counterpart on ß-arrestin-2 or using a specific TAT-P1 peptide to block the interaction between ß-arrestin-1 and PLCγ abolishes TRV120027-induced TRPC3 activation. Taken together, our results show that the GPCR-arrestin complex initiates non-desensitized signalling at the plasma membrane by coupling with ion channels. This fast communication pathway might be a common mechanism of several cellular processes.
Subject(s)
Catecholamines/metabolism , Receptor, Angiotensin, Type 1/agonists , TRPC Cation Channels/metabolism , beta-Arrestin 1/metabolism , beta-Arrestin 2/metabolism , Animals , Calcium/metabolism , Estrenes/pharmacology , HEK293 Cells , Humans , Ligands , Mice, Knockout , Oligopeptides/pharmacology , Phospholipase C gamma/metabolism , Pyrrolidinones/pharmacology , Receptor, Angiotensin, Type 1/metabolism , Signal Transduction/drug effects , beta-Arrestin 1/chemistryABSTRACT
BACKGROUND: Free fatty acid 4 (FFA4) (GPR120) receptor functions as a receptor for unsaturated long-chain free fatty acids by regulating the secretion of glucagon-like peptide-1 and suppressing the inflammatory process, in which these two distinct biological functions are modulated by two signaling pathways, Gq and ß-arrestin2, respectively. RESULTS: By using pharmacophore modeling and virtual screening methods, several compounds are found with excellent activities for agonizing FFA4 receptor. It needs to be noted that among them, some molecules demonstrate appealing ß-arrestin2-biased properties for the FFA4 receptor. CONCLUSION: These compounds may serve as the useful toolkits for detecting differential biased mechanism and developing new candidate therapeutic agents of the FFA4 receptor.
Subject(s)
Arrestins/metabolism , Drug Discovery , Receptors, G-Protein-Coupled/agonists , Small Molecule Libraries/pharmacology , Drug Evaluation, Preclinical , Humans , Molecular Structure , Receptors, G-Protein-Coupled/metabolism , Signal Transduction/drug effects , Small Molecule Libraries/chemistry , beta-ArrestinsABSTRACT
Specific arrestin conformations are coupled to distinct downstream effectors, which underlie the functions of many G-protein-coupled receptors (GPCRs). Here, using unnatural amino acid incorporation and fluorine-19 nuclear magnetic resonance ((19)F-NMR) spectroscopy, we demonstrate that distinct receptor phospho-barcodes are translated to specific ß-arrestin-1 conformations and direct selective signalling. With its phosphate-binding concave surface, ß-arrestin-1 'reads' the message in the receptor phospho-C-tails and distinct phospho-interaction patterns are revealed by (19)F-NMR. Whereas all functional phosphopeptides interact with a common phosphate binding site and induce the movements of finger and middle loops, different phospho-interaction patterns induce distinct structural states of ß-arrestin-1 that are coupled to distinct arrestin functions. Only clathrin recognizes and stabilizes GRK2-specific ß-arrestin-1 conformations. The identified receptor-phospho-selective mechanism for arrestin conformation and the spacing of the multiple phosphate-binding sites in the arrestin enable arrestin to recognize plethora phosphorylation states of numerous GPCRs, contributing to the functional diversity of receptors.
Subject(s)
Arrestins/metabolism , Phosphoproteins/metabolism , Receptors, G-Protein-Coupled/metabolism , Animals , Arrestins/genetics , Binding Sites , Blotting, Western , Cattle , Clathrin/metabolism , Escherichia coli , Fluorine , Fluorine-19 Magnetic Resonance Imaging , G-Protein-Coupled Receptor Kinase 2/metabolism , G-Protein-Coupled Receptor Kinases/metabolism , HEK293 Cells , Humans , Microscopy, Confocal , Mutation , Nuclear Magnetic Resonance, Biomolecular , Phosphate-Binding Proteins/metabolism , Protein Conformation , Signal Transduction , Tandem Mass Spectrometry , Tyrosine/analogs & derivatives , Tyrosine/metabolism , beta-Arrestin 1 , beta-ArrestinsABSTRACT
The tyrosine phosphorylation barcode encoded in C-terminus of HER2 and its ubiquitination regulate diverse HER2 functions. PTPN18 was reported as a HER2 phosphatase; however, the exact mechanism by which it defines HER2 signaling is not fully understood. Here, we demonstrate that PTPN18 regulates HER2-mediated cellular functions through defining both its phosphorylation and ubiquitination barcodes. Enzymologic characterization and three crystal structures of PTPN18 in complex with HER2 phospho-peptides revealed the molecular basis for the recognition between PTPN18 and specific HER2 phosphorylation sites, which assumes two distinct conformations. Unique structural properties of PTPN18 contribute to the regulation of sub-cellular phosphorylation networks downstream of HER2, which are required for inhibition of HER2-mediated cell growth and migration. Whereas the catalytic domain of PTPN18 blocks lysosomal routing and delays the degradation of HER2 by dephosphorylation of HER2 on pY(1112), the PEST domain of PTPN18 promotes K48-linked HER2 ubiquitination and its rapid destruction via the proteasome pathway and an HER2 negative feedback loop. In agreement with the negative regulatory role of PTPN18 in HER2 signaling, the HER2/PTPN18 ratio was correlated with breast cancer stage. Taken together, our study presents a structural basis for selective HER2 dephosphorylation, a previously uncharacterized mechanism for HER2 degradation and a novel function for the PTPN18 PEST domain. The new regulatory role of the PEST domain in the ubiquitination pathway will broaden our understanding of the functions of other important PEST domain-containing phosphatases, such as LYP and PTPN12.
Subject(s)
Catalytic Domain , Protein Tyrosine Phosphatases, Non-Receptor/chemistry , Protein Tyrosine Phosphatases, Non-Receptor/metabolism , Receptor, ErbB-2/metabolism , Ubiquitination , Amino Acid Motifs , Amino Acid Sequence , Breast Neoplasms/metabolism , Breast Neoplasms/pathology , Cell Line, Tumor , Crystallography, X-Ray , Female , Humans , Hydrophobic and Hydrophilic Interactions , Kinetics , Lysine/metabolism , Lysosomes/metabolism , Models, Biological , Molecular Sequence Data , Neoplasm Staging , Peptides/metabolism , Phosphorylation , Phosphotyrosine/metabolism , Proteasome Endopeptidase Complex/metabolism , Proteolysis , Signal Transduction , Structure-Activity Relationship , Substrate Specificity , beta-Transducin Repeat-Containing Proteins/metabolismABSTRACT
Striatal-enriched tyrosine phosphatase (STEP) is an important regulator of neuronal synaptic plasticity, and its abnormal level or activity contributes to cognitive disorders. One crucial downstream effector and direct substrate of STEP is extracellular signal-regulated protein kinase (ERK), which has important functions in spine stabilisation and action potential transmission. The inhibition of STEP activity toward phospho-ERK has the potential to treat neuronal diseases, but the detailed mechanism underlying the dephosphorylation of phospho-ERK by STEP is not known. Therefore, we examined STEP activity toward para-nitrophenyl phosphate, phospho-tyrosine-containing peptides, and the full-length phospho-ERK protein using STEP mutants with different structural features. STEP was found to be a highly efficient ERK tyrosine phosphatase that required both its N-terminal regulatory region and key residues in its active site. Specifically, both kinase interaction motif (KIM) and kinase-specific sequence of STEP were required for ERK interaction. In addition to the N-terminal kinase-specific sequence region, S245, hydrophobic residues L249/L251, and basic residues R242/R243 located in the KIM region were important in controlling STEP activity toward phospho-ERK. Further kinetic experiments revealed subtle structural differences between STEP and HePTP that affected the interactions of their KIMs with ERK. Moreover, STEP recognised specific positions of a phospho-ERK peptide sequence through its active site, and the contact of STEP F311 with phospho-ERK V205 and T207 were crucial interactions. Taken together, our results not only provide the information for interactions between ERK and STEP, but will also help in the development of specific strategies to target STEP-ERK recognition, which could serve as a potential therapy for neurological disorders. Regulation of phospho-ERK by STEP underlies important neuronal activities. A detailed enzymologic characterisation and cellular studies of STEP revealed that specific residues in KIM and active site mediated ERK recognition. Structural differences between the KIM-ERK interfaces and the active site among different ERK phosphatases could be targeted to develop specific STEP inhibitor, which has therapeutic potential for neurological disorders. PKA, protein kinase A & NGF, nerve growth factor.
Subject(s)
Mitogen-Activated Protein Kinase 1/metabolism , Protein Tyrosine Phosphatases, Non-Receptor/metabolism , Amino Acid Sequence , Animals , Catalytic Domain , Models, Molecular , Molecular Sequence Data , Mutation , PC12 Cells , Phosphorylation , Protein Tyrosine Phosphatases, Non-Receptor/genetics , RatsABSTRACT
The heavy metal cadmium is a non-degradable pollutant. By screening the effects of a panel of metal ions on the phosphatase activity, we unexpectedly identified cadmium as a potent inhibitor of PPM1A and PPM1G. In contrast, low micromolar concentrations of cadmium did not inhibit PP1 or tyrosine phosphatases. Kinetic studies revealed that cadmium inhibits PPM phosphatases through the M1 metal ion binding site. In particular, the negative charged D441 in PPM1G specific recognized cadmium. Our results suggest that cadmium is likely a potent inhibitor of most PPM family members except for PHLPPs. Furthermore, we demonstrated that cadmium inhibits PPM1A-regulated MAPK signaling and PPM1G-regulated AKT signaling potently in vivo. Cadmium reversed PPM1A-induced cell cycle arrest and cadmium insensitive PPM1A mutant rescued cadmium induced cell death. Taken together, these findings provide a better understanding of the effects of the toxicity of cadmium in the contexts of human physiology and pathology.
Subject(s)
Cadmium/chemistry , Cadmium/pharmacokinetics , Models, Chemical , Phosphoprotein Phosphatases/antagonists & inhibitors , Phosphoprotein Phosphatases/metabolism , Binding Sites , Computer Simulation , Enzyme Activation , HEK293 Cells , Humans , Kinetics , Protein Binding , Protein Phosphatase 2CABSTRACT
<p><b>AIM</b>To develop a method for separating the major bile acids by capillary zone electrophoresis (CZE).</p><p><b>METHODS</b>The effect of different separations, such as the compose, pH and the concentration of buffer, on the electro-osmotic flow (EOF), the migration time and resolution of 8 bile acids in this system were studied. The general trends in migration time could be correlated to the pH and concentration of the buffer. The effect of organic reagent on EOF and migration time were also investigated. By addition of methanol, the EOF went smaller than before, and better resolution was achieved. The experimental results showed that optimum separation was achieved under the following condition: buffer composition of 126 mmol.L-1 disodium tetraborate, 43 mmol.L-1 disodium hydrogenphosphate, 18% methanol; temperature 30 degrees C; voltage 30 kV; total length of capillary 570 mm and 500 mm from injection end; ultraviolet detection at 200 nm; pressure injection 5 kPa for 8 s.</p><p><b>RESULTS</b>Eight kinds of bile acid had been separated by CZE with only one injection. The method was used to analyse the contents of bile acids from different kinds of bear biles, the recovery was 89%-107%.</p><p><b>CONCLUSION</b>This method is simple and rapid, and can be used to determine the content of bile acids in bear biles. The calibration curve showed good linearity for eight bile acids in the concentration range of 4-60 mg.mL-1 (gamma > 0.9954). The total time for seperation and determination was within 25 min.</p>
