Your search keyword '"Leykam J"' showing total 2 results

1. Purification and characterization of a novel physiological substrate for calcineurin in mammalian cells.

Author

Groblewski GE, Yoshida M, Bragado MJ, Ernst SA, Leykam J, and Williams JA

Subjects

Amino Acid Sequence, Animals, Base Sequence, Calcineurin Inhibitors, DNA, Edetic Acid pharmacology, Humans, Immune Sera, Immunosuppressive Agents pharmacology, Molecular Sequence Data, Okadaic Acid pharmacology, PC12 Cells, Phosphoproteins genetics, Phosphoproteins metabolism, Phosphorylation, Rats, Rats, Sprague-Dawley, Sequence Homology, Amino Acid, Serine metabolism, Substrate Specificity, Calcineurin metabolism, DNA-Binding Proteins, Phosphoproteins isolation & purification, Transcription Factors

Abstract

Although the calcium/calmodulin-regulated protein phosphatase calcineurin has been shown to play a role in a number of intracellular processes, relatively few of the downstream phosphoproteins that are dephosphorylated by this enzyme in cells have been described. Calcineurin was previously shown to play a role in amylase secretion by rat pancreatic acinar cells and to specifically dephosphorylate a 24-kDa cytosolic protein. The present study describes the purification and characterization of this novel phosphoprotein, termed CRHSP-24 (calcium-regulated heat-stable protein with a molecular mass of 24 kDa). Microgram quantities of CRHSP-24 were purified from a large-scale rat pancreas preparation in a procedure involving heat and acid precipitation, anion-exchange chromatography, preparative electrophoresis, electroelution, and two-dimensional electrophoresis. Internal amino acid sequence was obtained from two peptides following trypsin digestion and high pressure liquid chromatography. Both sequences matched with 100% identity nucleotide sequences of expressed sequence tags from human placenta and rat PC-12 cells. Two CRHSP-24 transcripts of 0.7 and 2. 9 kilobases were detected in multiple rat tissues by Northern analysis, whereas a single 24-kDa protein was observed by Western blotting. The CRHSP-24 protein is 147 amino acids in length, is composed of nearly 14% proline, and is phosphorylated entirely on serine residues. Western analysis and 32P metabolic labeling of acini revealed CRHSP-24 to be maximally phosphorylated in control cells and to undergo a rapid sustained dephosphorylation on at least 3 serine residues in response to calcium-mobilizing stimuli. Dephosphorylation of CRHSP-24 was completely inhibited by pretreatment of acini with cyclosporin A or FK506. Furthermore, the inhibitory effects of FK506 were blocked by excess rapamycin. The ubiquitous expression of CRHSP-24 in rat tissues suggests that this novel calcineurin substrate plays a common role in calcium-mediated signal transduction.

Published

1998

2. An approach to locate phosphorylation sites in a phosphoprotein: mass mapping by combining specific enzymatic degradation with matrix-assisted laser desorption/ionization mass spectrometry.

Author

Liao PC, Leykam J, Andrews PC, Gage DA, and Allison J

Subjects

Amino Acid Sequence, Animals, Cattle, Chromatography, High Pressure Liquid methods, Lasers, Molecular Sequence Data, Peptide Fragments isolation & purification, Peptide Mapping, Phosphopeptides chemical synthesis, Phosphoproteins metabolism, Phosphorylation, Sensitivity and Specificity, Caseins chemistry, Mass Spectrometry methods, Peptide Fragments chemistry, Phosphopeptides chemistry, Phosphoproteins chemistry

Abstract

A rapid, picomole-scale method is described to locate phosphorylation sites in phosphoproteins by using matrix-assisted laser desorption/ionization time-of-flight mass spectrometry (MALDI-TOF-MS) combined with enzymatic modification of the analyte. There are three steps to locate phosphorylation sites in a phosphoprotein: (i) degradation of the phosphoprotein into small peptides by specific enzymatic or chemical reactions; (ii) identification of the phosphopeptides by -80 (or multiples of -80)-Da mass shifts in the mass spectra after dephosphorylation with alkaline phosphatase; (iii) location of the phosphorylation sites by mass mapping. As the size of the protein increases, it is advantageous to fractionate the mixture by HPLC and analyze each fraction by MALDI-TOF-MS. To perform mass mapping, the primary structure of the protein must be known. Bovine beta-casein was analyzed by this method. The conclusions about the specific phosphorylation sites of bovine beta-casein from our data coincide with previously reported results. From calculations, it is found that a mass spectrometer with 0.1% mass accuracy is sufficient, for mass mapping, to identify completely or partially digested tryptic peptides in the mass range of 100-8000 Da from bovine beta-casein (MW 23,983).

Published

1994