Evidence for N-Terminal Myristoylation of Tetrahymena Arginine Kinase Using Peptide Mass Fingerprinting Analysis

In this study, we confirmed N-terminal myristoylation of Tetrahymena pyriformis arginine kinase (AK1) by identifying a myristoylation signal sequence at the N-terminus. A sufficient amount of modified enzyme was synthesized using an insect cell-free protein synthesis system that contains all of the...

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Bibliographic Details
Published inProtein Journal Vol. 35; no. 3; pp. 212 - 217
Main Authors Motomura, Shou, Suzuki, Tomohiko
Format Journal Article
LanguageEnglish
Published New York Springer US 01.06.2016
Springer
Springer Nature B.V
Subjects
Amino Acid Sequence
Analysis
Animal Anatomy
Arginine
Arginine Kinase - chemistry
Biochemistry
Bioorganic Chemistry
Chemistry
Chemistry and Materials Science
Enzymes
Fatty acids
Histology
Kinases
Morphology
Myristic Acid - analysis
Organic Chemistry
Peptides
Peptides - chemistry
Protein biosynthesis
Protein synthesis
Protozoan enzymes
Tetrahymena
Tetrahymena pyriformis
Tetrahymena pyriformis - chemistry
Tetrahymena pyriformis - cytology
Tetrahymena pyriformis - enzymology
Peptide mass fingerprinting
Myristoylation
Arginine kinase
Subcellular localization
Tetrahymena pyriformis
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Summary:In this study, we confirmed N-terminal myristoylation of Tetrahymena pyriformis arginine kinase (AK1) by identifying a myristoylation signal sequence at the N-terminus. A sufficient amount of modified enzyme was synthesized using an insect cell-free protein synthesis system that contains all of the elements necessary for post-transcriptional modification by fatty acids. Subsequent peptide mass fingerprinting (PMF) analyses were performed after digestion with trypsin. The PMF data covered 39 % (143 residues) of internal peptides. The target N-myristoylated peptide had a theoretical mass of 832.4477 and was clearly observed with an experimental mass ( m/z -H + ) of 832.4747. The difference between the two masses was 0.0271, supporting the accuracy of identification and indicating that the synthesized T. pyriformis AK1 is myristoylated. The fixed specimens of T. pyriformis were reacted with an anti-AK1 peptide antibody followed by a secondary antibody with a fluorescent chromophore and were observed using immunofluorescence microscope. In agreement with previous western blotting analyses, microscopic observations suggested that AK1 is localized in the cilia. The present PMF and microscopic analyses indicate that T. pyriformis AK1 may be localized and anchored to ciliary membranes via N-terminal myristoyl groups.
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ISSN:1572-3887
1573-4943
1875-8355
DOI:10.1007/s10930-016-9663-0