Separation of Organic Acids in Plant Tissue by HPLC with a Twin Phase,Ion Exchange and Reverse Phase,Column

Abstract

No single isocratic chromatographic technique allows the complete separation of common organic aliphatic and alicyclic acids of plants. In order to obtain a better isocratic separation with a single HPLC method we combined in one chromatography assay the Ion Exchange and Reverse Phase technics in building a twin phase column. The first attempts are promising. This double chromatography based on the polarity of molecule (Reverse Phase) and on its acidic characteristics (Ion Exchange) has the advantages of both methods and allows good separations of the acids.     

High-Performance Liquid Chromatography of 2′-5′Oligoadenylates and Related Oligonucleotides

Abstract

HPLC has been used for the analysis and separation of the components of p_x (A2′p)_n A (x = 1 to 3, n = 1 to ≥4). Weak anion exchange columns give excellent resolution, but their instability in phosphate buffers makes them impractical for routine use. Reverse phase chromatography using C18 columns provides a satisfactory alternative method. For preliminary analysis of crude material, ammonium phosphate pH7.0 with a linear 1:1 methanol/H₂O gradient gives a good basic separation of the individual oligomers. Resolution of the 5′ mono-, di-and triphosphorylated oligomers or of the nonphosphorylated components can be obtained using ammonium phosphate pH6.0 and potassium phosphate pH6.5 buffers respectively. The C18 columns are very stable and any one column will give retention times reproducible within 0.2%.     

High Pressure Liquid Chromatographic Determination of Parabens in Pharmaceutical Preparations Containing Hydroxyquinolines

Abstract

A high pressure liquid chromatographic (HPLC) procedure for the analysis of methyl paraben (MP) and propyl paraben (PP) in pharmaceutical preparations containing a halogenated hydroxyquinoline (HHQ) is described. The method involves a separation of the phenolic constituents, MP, PP and HHQ with a Bio-Rad AG 1–X8 anion exchange resin, elution of the phenols with methanol after acidification and a reverse phase HPLC separation of the parabens using methanol-pH 6.5 buffer (60/40) mobile phase, a 30 cm × 3.9 mm (i.d.) column packed with Waters μBondapak C₁₈ packing and a guard column packed with Waters Bondapak C₁₈/Corasil packing. Recovery, precision, specificity and interference data along with the application of the proposed method for some commercial formulations both with and without a hydroxyquinoline are described.     

Quantitative Analysts of 5-Hydroxytryptamtne in Biological Material by High Perfornance Liquid Chromatography and Electrochmical Detection

Abstract

A quantitative method for the analysis of 5-hydroxytryptamine in biological material is described. The method is based on high performance liquid chromatography (HPLC) with electrochemical detection. A simple purification on a weakly acidic ion exchange resin prior to the analysis gives quite clean samples and permits concentration of diluted samples. The chromatographic separation is performed on a reverse phase column with organic modifier added to an aqueous eluent. With this analytical system 25 pg of 5-hydroxytryptamine can be detected.     

Separation of Xanthine Derivates by High Pressure Liquid Chromatography and Application to Plasma Analysis

Abstract

High pressure liquid chromatography (HPLC) methods were developed for separation and plasma analysis of ten xanthine derivates. Separation was evaluated on silica column and on three different reverse phase columns, with optimum conditions obtained on C₆ spherisorb column using isocratic elution with phosphate buffer 10^?2 M, pH 2.7 - acetonitrile mixture (80/20 V/V). Determination of these xanthine derivates in plasma for therapeutic control was studied.     

Determination of Cytokinins by Ion Suppression-Reverse Phase High Performance Liquid Chromatography

Abstract

A method for the separation of cytokinins has been developed by the use of ion suppression-reverse phase high performance liquid chromatography (IS-RP HPLC) with high efficiency, specificity and low sensitivity. Four reverse phase chromatographic columns were compared for their ability to separate and quantify six cytokinins with respect to signal response, resolution (R_S), capacity factor (k¹) and efficiency, N (number of theoretical plates). The optimal aqueous and organic phase components for the resolution of these cytokinins were determined with respect to pH, ionic strength and the proportion of the organic solvents, methanol and acetonitrile. Heptane sulfonic acid was used as an organic modifier. The optimal HPLC operating conditions were applied to separate and quantify the cytokinins present in a culture supernatant of Azotobacter chroococcum.     

Paired-Ion High Pressure Liquid Chromatography of Methotrexate and Metabolites in Biological Fluids

Abstract

A paired-ion high pressure liquid chromatography procedure (HPLC) is described for the separation of methotrexate and its major metabolites (7-hydroxymethotrexate, 4-amino-4-deoxy-N^lO-methylpteroic acid, methotrexate diglutamate, methotrexate triglutamate), and therapy-related compounds (Diamox and 5-methyltetrahydrofolate). The mobile phase consisted of a 70% solution of 5 mM hexanesulfonic acid, pH 3.75, and 30% methanol eluted on a reverse phase column or columns and monitored at 305 nm or 280 nm UV absorption. The lower limit of sensitivity for methotrexate and 7-hydroxymethotrexate in plasma was 2 ng/ml.     

A Simple Liquid Chromatographic Method for Analysis and Isolation of the Unsaturated Components of Anacardic Acid

Abstract

Good analytical and preparative separation of the saturated, monoene, diene and triene components of anacardic acid have been achieved by reverse phase HPLC on a C₁₈ column by isocratic elution with methanol-aqueous acetic acid.     

Separable Forms of Radioiodinated Ovine Lutropin (oLH) Subunits,Fractionated by Anion Exchange High Performance Liquid Chromatography and Analyzed by Radioimmunoassay

Abstract

Radioiodinated oLH α and oLH ß subunits were fractionated with the aid of high performance liquid chromatography (HPLC) using a Waters Protein Pak DEAE 5PW anion exchange column. The content of these subfractions differed in their binding maxima to their respective subunit antisera. An increase of the pH from 6.5 to 7.5 and 8.5 affected the chromatographic profile of 8-week-old radioiodinated α-subunit. Overall, material from the various radioactive peaks exhibited binding to ß-subunit antiserum in the range of 32.0% - 81.0%, depending on the storage time of the tracer and the pH. Shifting strategies, we either applied the labelled subunits to a Pharmacia gel filtration column or subjected them to cellulose adsorption prior to HPLC. The radioiodinated α- and β-subunits subjected to HPLC after gel filtration were both eluted in only one peak with respective immunoreactivities of 46.6% and 73.2%.

When radioiodinated β-subunit was applied first to a cellulose column and then to HPLC, the chromatographic profile showed two radioactive peaks with retention times of 5 min (73.2% immunoreactivity) and 7.5 min (43.0% immunoreactivity), respectively.

It was concluded that an 8-week-old-tracer i s useful in such studies, owing to its highly stable immunoreactivity after repurification on an anion exchange HPLC.     

Ion Exchange High Performance Liquid Chromatography of Leukotrienes

Abstract

A novel anion exchange liquid chromatographic system has been developed for isocratic separation of leukotrienes. Hydrophobic as well as ionic forces were found to influence the separation. By optimization of solvent strenght, ionic strenght and pH, amphoteric peptidoleukotrienes could be separated simultaneously with hydroxy fatty acids such as leukotriene B₄ and its ω-oxidized metabolites. To obtain a good buffering capacity of the mobile phase at optimum pH, a multicomponent buffer was developed.     

The Purification of Xanthene Dyes by Reverse Phase High Performance Liquid Chromatography

Abstract

A reliable method for the separation of fluorescein dyes from their impurities was developed using high performance liquid chromatography and involved a μBondapak C₁₈ reverse phase column and mixtures of methanol and ammonium acetate buffer. This technique was used to verify the purity of commercial products as well as to aid in the development of an empirical theory related to retention of halogenated fluorescein dyes by reverse phase columns.     

Purification of Human Platelet Monoamine Oxidase B by High Performance Liquid Chromatography

Abstract

Human platelet monoamine oxidase (MAO B), a membrane bound enzyme was purified to homogeneity by DEAE-Sephacel column chromatography, chromatofocusing, and high performance liquid chromatography (HPLC). The crucial purification step was HPLC on a anion exchange column (SynChropak AX 300). The HPLC column was eluted initially with potassium phosphate buffer (100 mM, pH 7.4) for 10 min at a flow rate of 1.0 ml/min, followed by a gradient (0–1%) of octyl-β-D-glucopyranoside (octylglucoside) in the same buffer for 10 min, and finally with buffered octylglucoside (1%) for 40 min. The elution of pargyline-bound or active MAO was established by determining either radioactivity in each fraction when MAO B had previously been covalently labeled with [³H]-pargyline [³H(G)] or catalytic activity using [¹⁴C-methylene]-benzylamine as substrate. [³H]-pargyline-bound and active MAO B eluted from the column at approximately 34 min. The extent of homogeneity and the subunit M_r (approximately 59,000) of MAO B were determined by sodium-dodecyl sulfate polyacrylamide gel electrophoresis followed by silver staining for proteins.     

Reverse Phase HPLC Determination OF 5,6-Dihydro-5-azacytidine in Biological Fluids

Abstract

A sensitive and specific reverse phase HPLC method which allows measurement of the new antitumor agent 5,6-dihydro-5-azacytidine (DHAC) in biological fluids at concentrations as low as 50 ng/ml (2 × 10^?7 M) has been developed. After addition of 5′-chloro-5′-deoxy-5,6-dihydro-5-azacytidine as an internal standard, sequential ultrafiltration, boronate gel affinity chromatography and cation exchange chromatography are employed to isolate DHAC from plasma or urine. DHAC is then reacted with N,N-dimethylformamide diethylacetal to form a dimethylaminomethylene derivative with enhanced UV detectability (λmax = 264 nm, log ε = 4.3) and better retention on a reverse phase column. Isocratic separation is then accomplished on a fully loaded and end-capped ODS column with 0.050 M formic acid in 20% acetonitrile/water. This assay has been used to determine the plasma pharmacokinetics of DHAC in rats given a single i.v. bolus dose of 50 mg/kg. Analysis of the drug in human plasma indicates that this method is suitable for determining DHAC disposition and pharmacokinetics in human subjects.     

Improved High Performance Liquid Chromatographic Method for the Quantification of 3-Methylhistidine in Serum and Urine

Abstract

We optimized an high-performance liquid chromatographic (HPLC) method for the determination of 3-methylhistidine (3-MeHis) in biological fluids. After pre-column derivatization with OPA, analytical separation was achieved on a reversed-phase C18 column by a simple gradient between sodium propionate buffer and acetonitrile. the method is accurate, reproducible and sensitive, and allows the determination of urinary 3-MeHis levels in about 55 min. Other additional 16 amino acids may be easily quantified while the 3-MeHis peak is well resolved from an unknown urinary compound potentially interfering.     

Purification of Radio-Iodinated Cholecystokinin Peptides by Reverse Phase HPLC

Abstract

The purification of the iodinated tracers of CCK peptides using Sphadex G5O chromatography does not allow for a good separation between non-modified peptides and labelled peptides. We present, in this paper a simple and rapid purification method using reverse phase HPLC with a C-18 column for four of these tracers. The biological characteristics of the molecules obtained demonstrate their strong specific radioactivity and their high degree of purity.     

Microdetermination of Bile Acids by High-Performance Liquid Chromatography Equipped with a High Sensitive Conductance Detector

Abstract

Conductimetric detection of bile acids in reversed phase high-performance liquid chromatography is described. The solvent system of the mixture of water and organic solvent containing small amount of basic salts such as ammonium carbonate is found useable by removing the cation with the cation exchange column inserted between the ODS column and the conductance detector. Thus, a few ng of tauro-and glyco-conjugated bile acids can be detected without tedious derivatization and hydrolysis.     

Preservation of Biological LH and FSH Activity after Application on HPLC. Comparison between Cation-Exchange and Reverse-Phase High Performance Liquid Chromatography

Abstract

A cation-exchange high-performance liquid chromatography procedure is described for the separation of bioactive lutropin from follitropin in a human urinary gonadotropin standard preparation (1st IRP 70/45). The results clearly demonstrate that recovered protein retained most of its biological activity following the chromatography. Due to a lack of efficient and quick methods for purifying pituitary or urinary gonadotropins, this method could prove to be valuable for this purpose. This method has also been shown to be quick (less than 20 min) and efficient for separation of impurities or degradation products from bovine follitropin with 92% preservation of its biological activity. Our results suggest that ion exchange HPLC procedure will play a powerful role in the isolation of gonadotropins and other biologically active compounds.     

Application of Thin Layer,Ion Exchange and High Performance Liquid Chromatography to Separate Pharmacologically Active Components of an African Arrow Poison of Plant Origin

Abstract

We have applied thin layer chromatography (TLC), ion exchange chromatography (IEC) and, high performance liquid chromatography (HPLC) to separate and identify the pharmacologically active components of an african arrow poison of plant origin. On the basis of Rf values obtained from TLC, the active components of the toxin are unlike d-tubocurarine, atropine and, scopolamine. Dowex 1 × 2 IEC of 630 mg of crude toxin on a 2.5″ × 33″ column with step gradient elution (NaCl, 0.1 - 1. OM and NaOH, 0.1M) led to the identification of three distinct peaks. When the components of each of the three peaks were subjected to HPLC, the results confirmed the homogeneity of each of the isolated peaks except for the third peak which was a doublet.     

Determination of antimony species with high-performance liquid chromatography using element specific detection

A new method for the fast and simultaneous determination of Sb(III) and Sb(V) is presented involving the use of anion exchange high-performance liquid chromatography (HPLC), a complexing reagent in the mobile phase, and element specific detection with flame atomic absorption spectrometry (FAAS) or inductively coupled plasma mass spectrometry (ICP-MS). Chromatographic parameters such as nature and concentration of the complexing and eluting compounds and pH of the mobile phase were investigated in detail. Additionally, the separation of inorganic Sb(III) and Sb(V) from organically bounded antimony (as (CH₃)₃SbCl₂ and (CH₃)₃Sb(OH)₂) was investigated by using anion, and cation exchange, and reversed phase HPLC. Best separation was obtained with anion exchange HPLC under alkaline conditions. Cation exchange and reversed-phase HPLC were not useful for the separation of the above compounds. With FAAS concentrations in the upper mg L^–1 range are detectable, which is not sensitive enough for the analyses of environmental samples. When the chromatographic system was coupled to ICP-MS, the detection limits are in the lower μg L^–1 range. The method was applied to various environmental samples with anthropogenic and naturally elevated Sb concentrations.     

Anion Exchange-Adsorption on Low Capacity Anion Exchangers: Separation of Organic Acids,Amino Acids,Small Chain Peptides

Abstract

The variables that influence the retention of organic analyte anions on a macroporous, high surface area polystyrenedivinyl-benzene copolymer that is chemically modified by attaching tetraalkylammonium groups to the copolymer surface are identified and studied as a function of anion exchange capacity. A combined adsorption-anion exchange retention of the organic analyte anion is possible providing the analyte has both a hydrophophic center and an anionic charge site. As the column anion exchange capacity (0 to 173 μeq of anion exchange sites/column was studied) increases, analyte retention due to adsorption decreases and retention due to anion exchange increases. The factors influencing organic analyte anion retention by adsorption are low anion exchange capacity and mobile phase solvent composition, type of organic modifier, and pH for analytes that are weak organic acids. For anion exchange the major factors are a high anion exchange