Rapid reverse phase-HPLC assay of HMG-CoA reductase activity.

Radioisotope-based and mass spectrometry coupled to chromatographic techniques are the conventional methods for monitoring HMG-CoA reductase (HMGR) activity. Irrespective of offering adequate sensitivity, these methods are often cumbersome and time-consuming, requiring the handling of radiolabeled chemicals or elaborate ad-hoc derivatizing procedures. We propose a rapid and versatile reverse phase-HPLC method for assaying HMGR activity capable of monitoring the levels of both substrates (HMG-CoA and NADPH) and products (CoA, mevalonate, and NADP+) in a single 20 min run with no pretreatment required. The linear dynamic range was 10–26 pmol for HMG-CoA, 7–27 nmol for NADPH, 0.5–40 pmol for CoA and mevalonate, and 2–27 nmol for NADP+, and limit of detection values were 2.67 pmol, 2.77 nmol, 0.27 pmol, and 1.3 nmol, respectively.


HPLC analysis
A HPLC system Gold (Beckman Coulter Inc.) equipped with a UV/VIS detector and HPLC column heater (Alltech) was used for the analysis. Reaction mixture consisting of HMGR (0.4 µM), NADPH (2.68 mM), and HMG-CoA (1.55 µM) diluted in the activity buffer was incubated at 37°C, and aliquots were withdrawn at indicated times and separated by HPLC. Each species (both isolated analytes and incubation mixtures) were injected and separated on a reverse phase Phenomenex Luna C18 column (5 m particle size, 250 × 4.6 mm equipped with a 5 mm guard column of the same phase), and thermostated at 26°C, with the following linear gradient of potassium phosphate 100 mM (solvent A) and methanol (solvent B): 10%-30% B up to 15 min and 30%-10% B for 5 min at fl ow rate of 0.8 ml/min, UV/VIS detector set at 260 nm. An injection volume of 10 l was used throughout. After each chromatographic elution, column was regenerated with two column volumes of 60% methanol. HMG-CoA, NADPH, and NADP + were directly monitored, whereas mevalonate was determined by monitoring CoA production (mevalonate/CoA 1:1 stoichiometric ratio; Fig. 1 ). Enzyme catalytic activity was performed at 37°C in a 100 mM sodium phosphate buffer containing 1 mM EDTA, 10 mM DTT, 2% DMSO, and 1 mM magnesium sulfate, pH 6.8, following the reaction for different times of incubation. No interfering signal was detected upon injection of the activity buffer. Each analysis was repeated in quadruplicate. Detection Abstract Radioisotope-based and mass spectrometry coupled to chromatographic techniques are the conventional methods for monitoring HMG-CoA reductase (HMGR) activity. Irrespective of offering adequate sensitivity, these methods are often cumbersome and time-consuming, requiring the handling of radiolabeled chemicals or elaborate ad-hoc derivatizing procedures. We propose a rapid and versatile reverse phase -HPLC method for assaying HMGR activity capable of monitoring the levels of both substrates (HMG-CoA and NADPH) and products (CoA, mevalonate, and NADP HMG-CoA reductase (HMGR) is the enzyme that catalyze the four-electron reductive deacylation of HMG-CoA to CoA and mevalonate ( Fig. 1 ) ( 1 ). This reaction is the controlling step in the biosynthesis of sterols and isoprenoids ( 2, 3 ); hence, a large number of studies on the modulation of HMGR activity are continuously performed in the effort of developing new drugs in the treatment of hypercholesterolemic disorders ( 1 ).
Herein, as an alternative for laboratories with no access to the expensive LC/MS equipment, we propose a rapid and adequately sensitive HPLC-based method capable of monitoring both the levels of all the species involved in the equilibrium in a single analysis and the kinetics of HMGR-catalyzed reactions. quantifi ed according to the standard addition method ( 18 ); different amounts of the isolated enzyme (30-130 ng per mg of total proteins) were added to the reaction mixture (NADPH, HMG-CoA, and cell lysate, dissolved in the activity buffer) and detecting the product of CoA after 60 min. This mixture was finally centrifuged at 10,000 g for 10 min. These quantities were of the HMGR levels and activity in cell homogenate was carried out on human colon cancer cell line HCT116, previously shown to express HMGR ( 17 ). Cells were suspended in the activity buffer added with phenyl-methane-sulfonyl-fl uoride and tosylphenyl-alanyl-chloromethyl-ketone as proteases inhibitors and lysated using a insulin syringe. Total cellular enzyme levels were  The same method was successfully applied to a cellular lysate, reporting comparable chromatographic profi les without any signifi cant interfering compounds ( Fig. 3B ).
Multiple standard additions of the isolated enzyme to reaction mixture containing cell lysate showed a linear correlation between CoA/mevalonate produced and total enzyme. The measured concentration of the cellular active enzyme was 52 ± 2 ng/mg of total proteins ( Fig. 5 ), corresponding to 15.58 ± 0.48 units/mg cell protein, consistent with previously studies on tumor cells ( 9 ).
Finally, the proposed method was validated by comparison with a commercially available spectrophotometric assay kit (Cod. CS1090, Sigma-Aldrich), which provided comparable levels of HMGR in HCT116 cell lysates (14.8 ± 0.4 units/mg of total cell proteins).
In conclusion, this method could represent a useful tool for both rapid and low-cost routine assays of HMGR activity, and quantitation of all the species involved in the equilibrium.

RESULTS AND DISCUSSION
Calibration curves were established for each single analyte over adequate ranges of concentrations ( Fig. 2 ). Dynamic ranges of linearity for the individual samples (determined by simple linear regression analysis), along with limits of detection (LODs) and limits of quantifi cation (LOQs) (determined as ratio between 3 and 5 times the RMSE of the linear fi t and the slope of the calibration curve, respectively) are reported in Table 1 . The linearity of the standard curves was evaluated with a Chi-square 2 goodness-of-fi t test ( P > 0.05).
The substrates and the products of the enzymatic reaction were clearly and completely separated from each other, as shown in Fig. 3A .
Time course of mevalonate/CoA production was analyzed according to a mono-exponential model ( Fig. 4 ), and bi-exponential analysis did not signifi cantly improve the quality of the fi t, as assessed with F-Test (95% confi dence).
The assay reproducibility was evaluated by comparison of intra-and inter-day variability over 5 days by performing four replicates each day, with maximum variation coeffi cient associated to peak area CV intra = 5.48% and CV inter = 6.31%, and to retention time CV intra = 0.14% and CV inter = 0.23%.   5. Linear dependence between isolated enzyme added and CoA/mevalonate produced in a cell lysate reaction mixture. Quantity of the enzyme present in the cell lysate (normalized by the total quantity of proteins) is derived from the intercept on the X-axis.