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Revision as of 03:09, 19 September 2015


Overview


Scroll down for more

Project

Introduction

Over the summer we worked with nonribosomal peptide synthetases (NRPSs). We developed a B. subtilis strain capable of oligo-mediated genome engineering and used this strain to alter a NRPS. We also investigated methods of screening for novel products with desired activities.

Background

Nonribosomal peptide synthases (NRPSs) are large multimodular enzymes that synthesize nonribosomal peptides, which are short bioactive peptides with a broad range of functions, including antibiotics, immunosuppressants and anticancer drugs.

MAGE subtilis

Multiplex automated genome engineering (MAGE) utilises cyclical recombination with short oligonucleotides in order to achieve a high allelic replacement efficiency and can be used to quickly generate cell populations with varying phenotypes. We introduced oligo-mediated genome engineering into Bacillus subtilis.

Surfactin

In order to verify that we could alter specificities of nonribosomal peptide synthetases to produce novel compounds, we used oligo-mediated recombineering to alter the surfactin peptide of B. subtilis.

Tyrocidine

Tyrocidine is a mixture of non-ribosomal peptides. It can only be used topically due to its toxicity. We sought to express the tyrocidine synthase cluster in B. subtilis to make novel derivatives with oligo-mediated recombineering.

Lab-on-a-disc

Lab-on-a-disc is a concept of a screening method for our MAGE method to distinguish bacterial colonies producing non-ribosomal peptides (NRPs) of interest. Simple technology and science behind this has a potential to screen a few bacterial cultures at the same time. 

Intein

When one method fails the Synthesizer team come up with a new idea! Alternative approach of generating short cyclized peptides with similar length to tyrocidine by using self-splicing proteins. Inteins are such short self-splicing proteins that have no function in the proteins they are a part of, besides catalyzing their own excision after translation. The splicing makes a peptide bond between the two adjacent amino acids next to the inteins.

Detection of NRP

Separation and identification of our non-ribosomal peptide synthetase (NRPS) products was determined by ultra-high performance liquid chromatography with diode array detection coupled to quadrupole time-of-flight mass spectrometry (UHPLC-DAD-QTOFMS). NRPS variants were identified by changes in mass/z and column retention time. 

Technical University of Denmark
Department of Systems Biology
Søltofts Plads 221
2800 Kgs. Lyngby
Denmark
P: +45 45 25 25 25
M: dtu-igem-2015@googlegroups.com