Richard E. Payne scite author profile

SummaryTwo hundred consecutive specimens received in this laboratory for "liver function tests" showed a wide range of abnormal protein concentrations. Calcium concentration correlated closely with albumin (r = 0867) but less closely with total protein (r = 0 682). A simple formula for adjusting calcium concentration was derived from the regression equation of calcium on albumin. Adjusted calcium = calcium -albumin + 4-0, where calcium is in mg/100 ml and albumin in g/100 ml.Low calcium concentrations were found in 49 (24-5%) and raised concentrations in six (3%) of the 200 blood specimens taken for liver function tests. After adjustment, the 95% limits of the observed range were identical with the 95%

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Albedo of the Sea Surface

Payne

1972

J. Atmos. Sci.

505

337

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The Cellular Distribution of Fluorescently Labeled Arrestins Provides a Robust, Sensitive, and Universal Assay for Screening G Protein-Coupled Receptors

Oakley¹,

Hudson

Cruickshank

et al. 2002

ASSAY and Drug Development Technologies

114

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G protein-coupled receptors (GPCRs) have proven to be a rich source of therapeutic targets; therefore, finding compounds that regulate these receptors is a critical goal in drug discovery. The Transfluor technology utilizes the redistribution of fluorescently labeled arrestins from the cytoplasm to agonist-occupied receptors at the plasma membrane to monitor quantitatively the activation or inactivation of GPCRs. Here, we show that the Transfluor technology can be quantitated on the INCell Analyzer system (INCAS) using the vasopressin V(2) receptor (V(2)R), which binds arrestin with high affinity, and the beta(2)-adrenergic receptor (beta(2)AR), which binds arrestin with low affinity. U2OS cells stably expressing an arrestin-green fluorescent protein conjugate and either the V(2)R or the beta(2)AR were plated in 96-well plastic plates and analyzed by the INCAS at a screening rate of 5 min per plate. Agonist dose-response and antagonist dose-inhibition curves revealed signal-to-background ratios of approximately 25:1 and 8:1 for the V(2)R and beta(2)AR, respectively. EC(50) values agreed closely with K(d) values reported in the literature for the different receptor agonists. In addition, small amounts of arrestin translocation induced by sub-EC(50) doses of agonist were distinguished from the background noise of untreated cells. Furthermore, differences in the magnitude of arrestin translocation distinguished partial agonists from full agonists, and Z' values for these ligands were >0.5. These data show that the Transfluor technology, combined with an automated image analysis system, provides a direct, robust, and universal assay for high throughput screening of known and orphan GPCRs.

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A New Look at Calibration and Use of Eppley Precision Infrared Radiometers. Part I: Theory and Application

Fairall¹,

Persson

Bradley

et al. 1998

J. Atmos. Oceanic Technol.

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The IMET (Improved Meteorology) Ship and Buoy Systems

Hosom¹,

Weller²,

Payne³

et al. 1995

J. Atmos. Oceanic Technol.

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Richard E. Payne

Interpretation of Serum Calcium in Patients with Abnormal Serum Proteins

Albedo of the Sea Surface

The Cellular Distribution of Fluorescently Labeled Arrestins Provides a Robust, Sensitive, and Universal Assay for Screening G Protein-Coupled Receptors

A New Look at Calibration and Use of Eppley Precision Infrared Radiometers. Part I: Theory and Application

The IMET (Improved Meteorology) Ship and Buoy Systems

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