Fast atom bombardment mass spectrometry and tandem mass spectrometry of biologically active peptidoglycan monomers from Neisseria gonorrhoeae.

S A Martin,R S Rosenthal,K Biemann

doi:10.1016/s0021-9258(18)47596-5

Abstract

Fast atom bombardment mass spectrometry (FABMS) and tandem mass spectrometry (MS/MS) were employed to define the structures of Neisseria gonorrhoeae peptidoglycan monomers that were of interest because of their abilities to mediate diverse biological reactions ranging from arthritogenicity to somogenicity. FABMS-determined molecular weights of individual components present in several different enzymatically derived classes of gonococcal monomers revealed that each of these classes was a complex mixture of up to 13 distinct peptidoglycan fragments. These ranged from the predominant disaccharide tetrapeptides possessing reducing or nonreducing 1,6-anhydro-N-acetylmuramic acid ends to relatively minor constituents containing glycine or asparagine in addition to traditional peptidoglycan amino acids, i.e. alanine, glutamic acid, and diaminopimelic acid. FABMS of high performance liquid chromatography-purified monomers yielded some sequence information; however, analysis even of unfractionated peptidoglycan mixtures using a JEOL HX110/HX110 tandem mass spectrometer operating at 10 kV provided unambiguous primary sequence data for the peptidoglycan monomers and defined the position of glycine in four compounds as well as the location of O-acetyl substituents (present on some compounds) on C-6 of the N-acetylmuramic acid residue.

Highlights

Fast Atom Bombardment Mass Spectrometry and Tandem Mass Spectrometry of Biologically Active PeptidoglycanMonomers from Neisseria gonorrhoeae”
Fast atom bombardment masspsectrometry (FABMS) andtandemmass spectrometry (MS/MS) were employed to define the structures of Neisseria gonorrhoeae peptidoglycan monomers that were of interest because of their abilities to mediate diverse biological reactions ranging from arthritogenicity to somnogenicity
FABMS of high performance liquid chromatographypurified monomersyielded some sequence information; analysis even of unfractionated peptidoglycan mixtures using a JEOL HX110/HX110 tandem mass spectrometer operating at 10 kV provided unambiguous primary sequence data for the peptidoglycan monomers and defined the position of glycine in fourcompounds as well as the location of 0-acetyl substituents on C-6 of the N-acetylmuramic acid residue

Summary

RESULTS

N . gonorrhoeae strain RD5 by FABMS prior to HPLC fractionationindicatedthe presence of several componentsin each preparation. Gonorrhoeae strain RD5 by FABMS prior to HPLC fractionationindicatedthe presence of several componentsin each preparation. The probability that all species in such a mixture could bedetected by FABMS dependson several factors. In mixtures in which the various species differ by single amino acids or minor structural modifications such ascyclization with corresponding loss of HzO, it is frequentlydifficult to ascertain whether thoebserved ion is a protonated molecular ion or a fragment ionof a molecule of higher mass. The latterpossibility is a prime consideration in the analysis of peptidoglycan monomers in which various structures differ by single amino acidsor sugar residues and/. Structures of Chalaropsis monomers (CM) and anhydrmorwmers (AMf)rom N. gonorrhoeae strain RD5 determined bvFAB MSIMS

Primary structure

SpecMtroamssetry of Peptidoglycan Monomers

DISCUSSION