Tetrachlorofluorescein TInsP as a Substrate Analog Probe for Measuring Phytase Activity in Surface Water: Proof of Concept.

An innovative approach for measuring phytase activity (PA) in surface water is presented. A substrate analog of -inositol hexakis(dihydrogen) phosphate (InsP), commonly referred to as phytic acid, 1--5--(1-oxo-1-(2' ,4,7,7' -tetrachloro-3',6'-dihydroxy-3-oxo-3H-spiro[isobenzofuran-1,9'-xanthen]-6-yl)-5,8,11-trioxa-2-azatridecan-13-yl)-inositol 1,2,3,4,6-pentakis--(dihydrogen) phosphate, referred to as tetrachlorofluorescein (TET) tethered (T)InsP, has been developed that can be used to monitor the (phytase-catalyzed) phosphate ester bond-cleavage reaction. Test phytases, (wheat [4-] and [3-] phytase) sequentially remove phosphate groups from TET TInsP, producing dephosphorylated probe species that were readily separated by reversed-phase high-performance liquid chromatography (RP-HPLC). Because dephosphorylated probe species retain the TET group, highly sensitive quantification could be achieved using fluorescence detection (excitation/emission ' = 245/540 nm). Calibration curves for TET TInsP, which could be used as a standard for quantifying all probe species, were linear ( > 0.999) over the range of concentrations tested. Phytase-generated dephosphorylated probe species were characterized or identified using RP-HPLC with mass spectrometry. Results of mass spectrometry analysis show that the RP-HPLC system was capable of distinguishing between dephosphorylated probe species at the regioisomeric level. The TET TInsP molecular probe was used to successfully measure PA in pond water. We found that the PA associated with the particulate plus water-soluble fraction was greater than that observed for the water-soluble fraction alone. Moreover, it appeared that 4- and 3-phytase were active in pond water based on an analysis of the chromatographic profile (i.e., elution sequence) of dephosphorylated probe species produced. The advent of a fluorescent substrate analog of InsP affords environmental scientists with the means to unambiguously quantify an extremely small amount of phytase-generated dephosphorylated product(s), enabling the measurement of PA over a reasonably short time duration, in an environmental sample containing low concentrations of enzyme.

Tethered phytic acid as a probe for measuring phytase activity.

A novel approach for measuring phytase activity is presented. We have developed a new chromophoric substrate analog of phytic acid, 5-O-[6-(benzoylamino)hexyl]-d-myo-inositol-1,2,3,4,6-pentakisphosphate that permits direct measurement of the phosphate ester bond-cleavage reaction using HPLC. This compound, along with its dephosphorylated T-phosphatidylinositol intermediates, are quantified using reversed phase chromatography with UV detection.

The fate of 14C-diazinon in compost, compost-amended soil, and uptake by earthworms.

A process for disposing of pesticide rinsates using sorption onto organic matter followed by composting is being evaluated. As a part of this evaluation process, we have studied the bioavailability of composted delta-2-14C-diazinon and its degradation products to earthworms (Eisenia foetida Savigny) in 30 and 60 d compost amended soil. After 60 d of composting there was considerable degradation of diazinon (95%) and a corresponding increase in the primary hydrolysis product, 2-isopropyl-4-methyl-6-hydroxypyrimidine (IMHP) as determined by high performance thin layer chromatography (HPTLC). Approximately 50% of the radioactivity became incorporated into the non-extractable fractions associated with composted organic matter with no measurable amounts of 14CO2 produced during the 60-day composting period. Following addition of the composted materials to soil, diazinon leading to 50% mortality after 14 d of exposure; continued to slowly degrade and become increasingly sorbed/entrapped within the soil-compost matrix. Soil amended with 30-d composted diazinon was toxic to earthworms whereas, no mortality was observed in those earthworms exposed to the 60-d composted diazinon. However, earthworms exposed to 30-d and 60-d composted diazinon were found to have similar levels of radioactivity in their tissues. The majority of the radioactivity in earthworms exposed 60-d composted diazinon was either unextractably bound within the earthworm tissue or was not acetone soluble. Most of the radioactivity that could be extracted with acetone was not separated by the two HPTLC methods we used. This study demonstrates that composting high concentrations of diazinon can greatly reduce toxicity and the amount of diazinon that is bioavailable to a representative soil macroinvertebrate (E. foetida).