Paula J. Johnson scite author profile

A simple method is described for the separation and quantification of the subunits of GSH transferases present in rat tissue extracts. This method, involving GSH-agarose affinity chromatography followed by reverse-phase h.p.l.c., is rapid and sufficiently sensitive to measure 5 micrograms of each subunit in a mixture. Examples are given of its application to extracts of rat kidney, adrenal, testicular interstitial cells and seminiferous tubules. The analysis of seminiferous tubules indicates that the technique may be of value for the identification of novel subunits. Preliminary separations of subunits from human GSH transferases are also described.

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Estimating thermodynamic properties of coal, char, tar and ash

Eisermann

Johnson

Conger

1980

Fuel Processing Technology

101

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Inter-laboratory ring trials to evaluate serological methods for dourine diagnosis

Cauchard¹,

Soldan

Madeline³

et al. 2014

Veterinary Parasitology

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Purification and Characterization of Phosphoribulokinase from the Marine Chromophytic Alga Heterosigma carterae1

Hariharan¹,

Johnson²,

Cattolico

1998

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In this study we characterized phosphoribulokinase (PRK, EC 2.7.1.19) from the eukaryotic marine chromophyte Heterosigma carterae. Serial column chromatography resulted in approximately 300-fold purification of the enzyme. A polypeptide of 53 kD was identified as PRK by sequencing the amino terminus of the protein. This protein represents one of the largest composite monomers identified to date for any PRK. The native holoenzyme demonstrated by flow performance liquid chromatography a molecular mass of 214 ؎ 12.6 kD, suggesting a tetrameric structure for this catalyst. Because H. carterae PRK activity was insensitive to NADH but was stimulated by dithiothreitol, it appears that the enzyme may require a thioredoxin/ferredoxin rather than a metabolite mode of regulation. Kinetic analysis of this enzyme demonstrated Michaelis constant values of ribulose-5-phosphate (226 M) and ATP (208 M), respectively. In summary, H. carterae PRK is unique with respect to holoenzyme structure and function, and thus may represent an alternative evolutionary pathway in Calvin-cycle kinase development.

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ASPEN modeling of the Tri-State indirect-liquefaction process

Begovich¹,

Clinton²,

Johnson³

et al. 1983

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Paula J. Johnson

The separation of glutathione transferase subunits by using reverse-phase high-pressure liquid chromatography

Estimating thermodynamic properties of coal, char, tar and ash

Inter-laboratory ring trials to evaluate serological methods for dourine diagnosis

Purification and Characterization of Phosphoribulokinase from the Marine Chromophytic Alga Heterosigma carterae1

ASPEN modeling of the Tri-State indirect-liquefaction process

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