New Procedure for Extraction of Ammonium from Natural Waters for 15N Isotopic Ratio Determinations

A new method for extracting ammonium from natural waters for ¹⁵N isotopic ratio determination is described. The method employs the conversion of the ammonium nitrogen into indophenol, which is then concentrated onto an octadecylsilane column. The method shows accuracy and precision comparable to those of other methods described in the literature. Some results from field experiments on the Swedish west coast are presented.     

An alternative procedure for the isolation of high mobility group proteins

A new procedure for the isolation of high mobility group proteins from chromatin is described. The method utilizes ammonium sulfate for both extraction and selective precipitation of the HMG proteins. It is rapid, simple, and provides high yields. The procedure has been used to obtain high mobility group proteins from rainbow trout and calf thymus chromatin.     

Nondenaturing procedure for rapid preparation of ferredoxin from Clostridium pasteurianum

A procedure is described for the rapid preparation of ferredoxin in high yield from crude extracts of C. pasteurianum. The method involves two successive chromatographic treatments on DEAE-cellulose in concentrated ammonium sulfate. Ferredoxin prepared by this method has an absorption spectrum and iron content similar to ferredoxin prepared by other methods.     

A Variation of the Pal Weigert Method for Staining Myelin Sheaths

A variation of the Pal-Weigert method for staining myelin sheaths is described, which is successful on some sections on which Pal's modification of the Weigert method fails; which does not require old ripened hematoxylin; and which can be completed in from three to five hours. It varies from the Pal-Weigert method by the insertion of a bath of ferric ammonium sulfate both before and after the staining with hematoxylin.     

Method for isolation of aminoacyl-tRNA synthetases from plants: purification and some properties of methionyl,phenylalanyl and arginyl tRNA synthetases from yellow lupin seeds

A method for the simultaneous purification of methionyl-, phenylalanyl- and arginyl-tRNA synthetases from yellow lupin seeds (Lupinus luteus) is described. The method uses ammonium sulphate fractionation, and DEAE-cellulose and DEAE-Sephadex A-50 column chromatography. Molecular weight and kinetic parameters of the pure enzymes are reported.     

Precipitation of phenyl and phenoxypenicillin from solutions using ammonium sulfate

An easy, rapid, and available method for separating 6-aminopenicillanic acid (6-APA), benzylpenicillin (penicillin G), and other related molecules from aqueous solutions or complex industrial broths is described. A high concentration of ammonium sulphate induces partially or totally the precipitation of the penicillin present in the solutions, while 6-APA, phenylacetic, and phenoxyacetic acid always remain in the supernatant. The filtration through No. 4 Pyrex glass-fiber filter or Whatman 3MM paper permits the separation of the compounds present in the supernatant from the other ones precipitated. The precipitated product was identified, in all cases, as ammonium penicillin. This method is described here for the first time.     

A high yield method for the isolation of sheep's liver cathepsin L

A method, giving twice the yield of the previous method, for the isolation of sheep's liver cathepsin L is described. The method uses three phase partitioning (TPP) in t-butanol/water/ammonium sulphate mixtures, followed by two chromatographic steps, at different pH values, in a single column of S-Sepharose.     

A sensitive method for the quantification of the mass of inositol phosphates using gas chromatography-mass spectrometry

A sensitive method to directly measure the mass of inositol phosphates from biologic samples is described. The procedure uses ammonium sulfate gradient elution anion exchange column chromatography to isolate inositol monophosphate, bisphosphate, trisphosphate, and tetrakisphosphate. The isolated fractions are dephosphorylated and subsequently desalted by a novel approach using solid barium hydroxide in a 1:1 stoichiometric ratio to the amount of ammonium sulfate present in the dephosphorylated sample. The myo-inositol derived from each inositol phosphate species was quantified by stable isotope dilution gas chromatography-mass spectrometry of the hexakis(trimethylsilyl) derivative using hexadeutero-myo-inositol as the internal standard. The applicability and sensitivity of this method are illustrated by measuring the mass of individual inositol phosphates in isolated adult canine cardiac myocytes.     

A new covalently modified support for gas-liquid phase sequencing

A new method for activation of glass fiber supports for immobilisation of proteins and peptides in gas-liquid phase sequencing is described. The new support offers several advantages over the presently used carrier polybrene: no precycling is required, initial yields are improved and background contamination is lower. This leads to an overall increase in detection sensitivity. The derivatisation method includes acid activation and subsequent covalent coating of glass fibers with quaternary ammonium groups thereby giving the glass surface a high binding capacity for both proteins and peptides. The activated glass has been successfully used for sequencing proteins and peptides isolated by HPLC as well as by electroelution from polyacrylamide gels.     

Isolation of high quality RNA from bilberry (Vaccinium myrtillus L.) fruit

A simple and efficient method is described for isolating high quality RNA from bilberry fruit. The procedure is based on the use of hexadecyltrimethyl ammonium bromide (CTAB), polyvinylpyrrolidone (PVP), and β-mercaptoethanol in an extraction buffer in order to eliminate the polysaccharides and prevent the oxidation of phenolic compounds. This method is a modification of the one described for pine trees, and yields high-quality RNA suitable for cDNA based methodologies. This method is applicable for a variety of plant tissues.     

Assay for soil urease activity

Summary A procedure is described that allows assay of soil urease activity. The method uses a phosphate buffer (pH 8.8) and a urea substrate concentration of 0.007 M. Incubation for 4 h at 37°C is recommended and urease activity is estimated by determining the amount of ammonium produced by urea hydrolysis in soil. The method is precise, and compares favourably with other procedures. re]19750710     

An improved histochemical method for measuring nitric oxide synthase activity

The previous quantitative histochemical method for measuring nitric oxide synthase (NOS) activity in tissue sections involved the loss of about 15 per cent of the NOS, presumably from the section into the reaction medium. Two changes are now described. The first is concerned with the preparation in the laboratory of the active reagent, lead ammonium citrate/acetate (LACA). The second change involves an improvement of the procedure for measuring NOS activity. The new method appears to retain all the measurable NOS activity inside the section. Copyright © 1999 John Wiley & Sons, Ltd.     

The prevention of distortion in ultrathin-layer polyacrylamide gel isoelectric focusing

Although isoelectric focusing patterns in ultrathin layers of polyacrylamide gel are distorted by the presence of salts, such as ammonium persulfate, this reagent is commonly used to promote polymerization of the gel. The amount of ammonium persulfate can be reduced but this causes the formation of sloppy gels or incomplete polymerization. A method is described here in which an ultrathin polyacrylamide gel is formed on a polyester sheet using ammonium persulfate in the absence of ampholyte. After complete polymerization, the ammonium persulfate is washed out and ampholyte is allowed to diffuse into the gel. Subsequent isoelectric focusing is then free from distortion caused by the presence of ammonium persulfate.     

A new and fast method for preparing high quality lambda DNA suitable for sequencing.

A method is described for the rapid purification of high quality lambda DNA. The method can be used from either liquid or plate lysates and on a small scale or a large scale. It relies on the preadsobtion of all polyanions present in the lysate to an "insoluble" anion-exchange matrix (DEAE or TEAE). Phage particles are then disrupted by combined treatment with EDTA/proteinase K and the resulting DNA is precipitated by the addition of the cationic detergent cetyl (or hexadecyl)-trimethyl ammonium bromide-CTAB ("soluble" anion-exchange matrix). The precipitated CTAB-DNA complex is then exchanged to Na-DNA and ethanol precipitated. The resultant purified DNA is suitable for enzymatic reactions and provides a high quality template for dideoxy-sequence analysis.     

Determination of ammonium ions in small urine volumes from laboratory animals

A method based on the indophenol reaction for the determination of ammonium ions in small urine samples from research animals is described. The method is precise and specific. Sensitivity (epsilon 630 molar = 174 X 10(3)) is far beyond needs. Interference by blood in hematuric samples can be avoided.     

Reduction of waste product excretion via nutrient control: Possible strategies for maximizing product and cell yields on serum in cultures of mammalian cells

Mammalian cells grown in culture excrete lactic acid and ammonium ions in quantities that may limit growth and reduce product synthesis. Frequent replenishment of the culture medium is often necessary to prevent waste product accumulation which could inhibit cell growth. Since increased medium replenishment results in increased usage of animal serum, the most expensive raw material, excessive production of waste products lowers the cell and product yield on serum, and hence increases production costs. Strategies for reducing the production of lactic acid and ammonium bymammalian cells via controlled addition of glucose and glutamine will be demonstrated. Mathematical relations coupling ammonium and glutamine kinetics will be described. Additionally, a method for automatic on-line estimation of the cell concentration was developed. This method involves calculating the ATP production rate from the oxygen uptake rate and the lactic acid production rate. Automatic online estimation of the cell concentration is critical if nutrient levels in large-scale mammaliancell cultures are to be accurately maintained via process control.     

Determination of Free Ammonium and Asparagine and Glutamine Amide-Nitrogen in Extracts of Plant Tissue

A relatively simple and rapid procedure for the measurement of free ammonium and the amides in plant extracts is described. The method was developed by combining a cation-exchange method for blood ammonia with a differential acid-hydrolysis procedure for asparagine and glutamine amide-nitrogen.The recovery of standard samples (100-400 mug of ammonium- or amide-nitrogen) of free ammonium, asparagine, and glutamine after being run through the extraction, column, and analytical procedures ranged between 99 and 102%.The harvest, extraction, and analytical procedures were tested on shoots from 4 to 6-day-old germinating barley seeds. The high levels of the amides and the low level of free ammonium present in the tissue extracts indicated that the extraction and analytical procedures resulted in little if any hydrolysis of the amides.     

A borate column for the separation of ribo and deoxyribonucleosides

A method is described for the separation of mixtures of the naturally occurring ribo- and deoxyribonucleosides by chromatography on columns of Dowex 50 eluted with ammonium borate. Nucleotides, ribonucleosides, and nucleotide-containing complex sugars are not retained on the column under these conditions, permitting unambiguous separation of these compounds from the deoxyribonucleosides, which are easily separated from each other by this chromatography. The elution positions of the nucleic acid bases allow partial to complete resolution from the corresponding deoxynucleosides. This column has either preparative or analytical utility for the procurement of nucleoside fractions free of the common contaminants.     

The substrate constant for the ammonium ion of growing

The relation between ammonium concentration and growth rate was studied in steady state continuous cultures of Saccharomyces cerevisiae in nitrogenlimited glucose ammonium medium. This relation could be described by the Monod equation. A maximum specific growth rate of 0.41 h^-1 and a substrate constant for ammonium of 5–11 M were calculated. Ammonium was determined by a modification of the phenol hypochlorite method. A discussion of the results in view of literature data on the substrate constants for other nutrients is given.