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Up to nine different products were detected by HPLC analysis; Reactions with metalloporphyrin/PhIO systems afforded high catalytic conversions (58 89%).
For qPCR gene expression analysis, reactions were performed in triplicate.
For sedimentation analysis, reactions were centrifuged at 16,100 g for 10 min at 25°C.
For MS-based analysis, reactions were quenched with four volumes of methanol and centrifuged to remove protein.
Real-time PCR was performed by mixing cDNA with primers, and iTaq™ Universal SYBR® Green Supermix quantitative PCR analysis reactions (Bio-Rad, USA).
HPLC analysis: Reactions were stopped with 0.1 ml of cold methanol and incubated with shaking (1000 rpm) for 5 min at 30°C to dissolve all available pyrethroids.
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The recombinant aromatase preparation was also characterized by reduced CO-difference spectral analysis, reaction product extraction assay, and inhibition studies using two aromatase inhibitors (letrozole and anastrozole).
Topics covered include chemical analysis, reaction kinetics, CO2 solubility, and innovative configurations of absorption and stripping columns as well as information on technology applications.
For the first-stage NTC behavior, five competing reactions were identified as being important based on sensitivity analysis, reaction pathway analysis, and simplified mechanism method.
The separation was used to optimize the derivatization conditions simultaneously for all the nucleobases in terms of pH, solvent system for reaction, amount of derivatizing reagent added per analysis, reaction time, and solvent for the extraction of the compounds.
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