Mass Spectrometric Analysis of Ehrlichia chaffeensis Tandem Repeat Proteins Reveals Evidence of Phosphorylation and Absence of Glycosylation 英文参考文献.docVIP
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Mass Spectrometric Analysis of Ehrlichia chaffeensis Tandem Repeat Proteins Reveals Evidence of Phosphorylation and Absence of Glycosylation 英文参考文献
MassSpectrometricAnalysisofEhrlichiachaffeensis
TandemRepeatProteinsRevealsEvidenceof
PhosphorylationandAbsenceofGlycosylation
AbdulWakeel1,XiaofengZhang1,JereW.McBride1,2,3,4,5*
1DepartmentofPathology,UniversityofTexasMedicalBranch,Galveston,Texas,UnitedStatesofAmerica,2DepartmentofMicrobiologyandImmunology,Universityof
Texas Medical Branch, Galveston, Texas, United States of America, 3Center for Biodefense and Emerging Infectious Diseases, University of Texas Medical Branch,
Galveston, Texas, United States of America, 4Sealy Center for Vaccine Development, University of Texas Medical Branch, Galveston, Texas, United States of America,
5InstituteforHumanInfectionsandImmunity,UniversityofTexasMedicalBranch,Galveston,Texas,UnitedStatesofAmerica
Abstract
Background: Ehrlichia chaffeensis has a small subset of immunoreactive secreted, acidic (pI ,4), tandem repeat (TR)-
containing proteins (TRPs), which exhibit abnormally large electrophoretic masses that have been associated with
glycosylationoftheTRdomain.
Methodology/PrincipalFindings:Inthisstudy,weexaminedtheextentandnatureofposttranslationalmodificationson
thenativeTRP47andTRP32usingmassspectrometry.Matrix-assistedlaserdesorption/ionizationtime-of-flight(MALDI-TOF)
demonstratedthatthemassofnativeTRP47(33,104.5Da)andTRP32(22,736.8Da)wereslightlylarger(179-and288-Da,
respectively)thantheirpredictedmasses.TheanomalousmigrationofnativeandrecombinantTRP47,andtherecombinant
TR domain (C-terminal region) were normalized by 1-ethyl-3-(3-dimethylaminopropyl)carbodiimide (EDC) modification of
negatively charged carboxylates to neutral amides. Exhaustive tandem mass spectrometric analysis (92% coverage)
performed on trypsin and Asp-N digested native TRP47 identified peptides consistent with their predicted masses. Two
TRP47peptidesnotidentifiedwerelocatedinthenormallymigratingamino(N)-terminalregionofTRP47andcontained
predicted phosphorylation sites (tyrosine and serine residues). Moreover, native TRP47 was immunoprecipita
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