Title page for ETD etd-11212000-132345


Type of Document Master's Thesis
Author Gilmore, Meghan Elizabeth
Author's Email Address mgilmore@vt.edu
URN etd-11212000-132345
Title Analysis of the Roles of the cwlD Operon Products during Sporulation in Bacillus subtilis
Degree Master of Science
Department Biology (Microbiology)
Advisory Committee
Advisor Name Title
Popham, David L. Committee Chair
Chen, Jiann-Shin Committee Member
Yousten, Allan A. Committee Member
Keywords
  • cortex
  • Bacillus subtilis
  • sporulation
  • peptidoglycan
Date of Defense 2000-11-15
Availability unrestricted
Abstract
CwlD has sequence similarities to N-acetyl muramoyl-L-alanine amidases, a class of enzymes known to cleave the bond between the

CwlD has sequence similarities to N-acetyl muramoyl-L-alanine amidases, a class of enzymes known to cleave the bond between the peptide side chain and the N-acetyl muramic acid residue in cortex peptidoglycan formation during sporulation. A major difference between vegetative peptidoglycan and spore peptidoglycan is the presence of muramic-d -lactam (MAL) in spore peptidoglycan. It was previously determined that a cwlD null mutant does not contain muramic-d -lactam in the spore cortex peptidoglycan and the mutant spores were unable to complete germination. Therefore, it is believed that CwlD plays a role in MAL formation during sporulation. However, the specific role of the protein had not been demonstrated. It was also previously found that cwlD is in a two-gene operon with orf1. Orf1 is produced within the forespore with CwlD. The hypothesized role of Orf1 is to inhibit CwlD activity from within the forespore.

Muramoyl-L-alanine amidase activity was demonstrated by CwlD in vivo. Therefore, CwlD is carrying out the first step of MAL synthesis, cleaving the peptide side chain while other enzymes are needed to complete MAL formation. Two different forms of CwlD were over-expressed, with and without the protein's signal peptide sequence. Both forms of the protein were purified and in both cases activity was undetectable. Antibodies specific for CwlD were obtained which can be used in future research as a tool to further characterize CwlD activity.

A series of B. subtilis cwlD operon mutants were constructed altering the expression patterns of Orf1 and CwlD within the mother cell and forespore compartments. Various resistance properties and the germination ability of the mutant dormant spores were analyzed. It was determined that the absence of just Orf1 or Orf1 and CwlD from within the forespore has no effect on the phenotypes tested. Peptidoglycan from developing mutant forespores was extracted and analyzed throughout sporulation. Evidence was obtained demonstrating that the role of Orf1 is not to inhibit CwlD from within the forespore as hypothesized.

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