the cyanobacteria group (cip)
DESCRIPTION
The cyanobacteria group (CIP) Laboratory of bacterial physiology and gggggggggggggggggggggg genetics. Dr Annick Wilmotte Dr Zorigto Namsaraev Rafael Fernandez Carazo Yannick Lara Pedro De Carvalho Maalouf Marie-José Mano - PowerPoint PPT PresentationTRANSCRIPT
The cyanobacteria group (CIP)Laboratory of bacterial physiology and
gggggggggggggggggggggg genetics
Dr Annick WilmotteDr Zorigto NamsaraevRafael Fernandez CarazoYannick LaraPedro De Carvalho MaaloufMarie-José ManoAlexandre LambionMarine Renard
Dr Olga Savichtcheva Magda Calusinska
Molecular taxonomy and evolution of cyanobacteria
I. The Centre for Protein Engineering
II. Earlier collaborations with SCK.CEN
III. Molecular diversity of cyanobacteria in diverse environments
A) Basis: Long-term interest for the diversity of the genus Arthrospira
B) Collaborations with SCK.CEN about MELiSSA
A) B-BLOOMS: toxic cyanobacterial blooms in Belgium
B) Discovery of the genotypic diversity of the cyanobacteria in the region of the New Belgian Antarctic Research Station ‘Princess Elisabeth’
C) BCCM collection of cyanobacterial strains from the Antarctic and Arctic
IV. Molecular ecology of Hydrogen production by Clostridia
II. Earlier collaborations with SCK.CEN
A) Basis: Long-term interest for the diversity of the genus Arthrospira1) The first paper proving that the genera Spirulina and Arthrospira are different , on the basis of their 16S rRNA2) two papers dealing with the diversity of 54 strains from 4 continents, based on a molecular taxonomy marker (ITS, spacer between the genes coding for 16S and 23S rRNA). The ITS was surprinsingly conserved, even for strains of different geographic origins.
Strain PCC 8005ITS-tree of 16 representative Arthrospira strains and old dried samples (up to 40 years old)
B) Collaborations with SCK.CEN about MELiSSA
MELiSSA Annual report 2004MELiSSA Annual report 2003
• 2002-4: MELGEN1 • Genetic stability of strain PCC8005, fingerprinting with AFLP, ‘Genome
Watch’
• 2005-9: AWM fellowship to Nicolas Morin• Genome of Arthrospira PCC8005 and effects of space-related stress
• 2008-9: MELGEN2 (1 year PhD fellowship to Karin Vauchel)• Genomic stability of Rhodospirillum rubrum S1• Genomic fingerprints with repeats: effects of high light intensities
OUTPUTS: REPORTS
Dr Max Mergeay & Natalie Leys, Laboratory of Molecular and Cellular Biology, Unit of Microbiology, Institute for Health, Environment and Safety
To solve questions on their phylogeny, diversity, ecological and geographical distribution, their potential for toxin production, their genetic stability
® Use of molecular taxonomic markers, as the ribosomal RNA sequences, spacers between 16S and 23S rRNA genes, house-keeping genes, Multiple Locus Sequence Analysis
®Techniques: PCR, Q-RT PCR, Whole Genome Amplification, Denaturating Gradient Gel Electrophoresis, Clone libraries, Genomic fingerprints, Whole genome Amplification, Bioinformatics
®Soon: next-generation sequencing 454
Microscopic organisms, with simple and variable morphologies microscopic observation is not adequate to study their diversity and evolution
III. Molecular diversity of cyanobacteria in diverse environments
Certain cyanobacterial taxa
- very resistant to dessication/radiation- UV protection mechanisms - tolerate high or low temperatures- tolerate high or low light intensities- tolerate high or low salinities- certain metabolic flexibility (anoxygenic photosynthesis,
heterotrophic capacity, nutrient scavenging)- N2 fixation
Limits? Low pH!
III. Molecular diversity of cyanobacteria in diverse environments
A) B-BLOOMS: toxic cyanobacterial blooms in BelgiumIn Belgium, toxic cyanobacterial blooms were observed in Flanders , Wallonia and Brussels. Microcystin concentrations exceded the threshold value of 25 ng/L (French directive for recreation waters)
Techniques used:Molecular diversity: DGGE of 16S rRNA/ITS, Clone libraries, Real time QPCR, Whole Genome Amplification on ‘single colonies’Toxigenicity: PCR for the operons synthetizing the toxins (when known)
Identification WoronichiniaPCR to detect operons for synthesis of secondary metabolites (NRPS, PKS)
Single colonies
B) Discovery of the genotypic diversity of the cyanobacteria in the region of Utsteinen in Antarctica (New Belgian Research Station Princess Elisabeth) Ridge
Belspo
Proxy for life on Mars?Collaboration with Prof. Javaux on the search for the signatures of Life
Diversity of cyanobacteria in the region of the Princess Elisabeth station
Characterisation of isolated strains
Leptolyngbya molecular diversity
0.05
E coli Z83204.1
PE-strain-13
clone China marine water S1-60 (EF491320)ё"еclone McMurdo desert H_21 (FJ490341)
PE0918b176
Lept. frigida ANT.LH52B.3 (AY493612)
PE34D1b2
clone McMurdo desert H_24 (FJ490344)
PE50cD5b PE50sD4b PE160D8b
PE0918b182 PE0946b148
Lept sp. ANT.RAUER8.1 (AY493619) Lept. sp. OU_6 Devon lime (GQ162217)
clone Lake Reid mat RJ088 (DQ181681) clone Lake Heart mat H-B09 (DQ181720)
clone Utah desert SD-F11 (EU751464) clone Tibetan desert QB63 (FJ790628) PE-strain-12 PE0918b167
100
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81
86
7898
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96
Characterisation of the community
DGGE gel
C) A BCCM collection of cyanobacterial strains from the Antarctic and Arctic
The Belgian Co-ordinated Collections of Micro-organisms has started an integration project for new collections, among which polar cyanobacteria (http://bccm.belspo.be/projects/programme2005-2008/c30014/). 125 unicyanobacterial strains are now included (http://www.cip.ulg.ac.be/newsite/pages/collectioncyano.php).
Contact: Annick Wilmotte ([email protected]) and Marine Renard ([email protected]), Centre for Protein Engineering, Institute of Chemistry B6, 4000 Liège, Belgium. Tel: 32 04 366 33 87, FAX: 32 4 366 33 64
1) Use of molecular ecology techniques to monitor the consortia of Clostridia producing H2, and their activities in the bioreactors
2) Study of the metabolic activity of the strains and expression of the different hydrogenases found by bioinformatic study of genomes
B FB 1
FB 2
FB 2
FB 3
FB 4
FB 4
FB 5
FB 6
0%
20%
40%
60%
80%
100%
% of H2ase transcripts C.pasteurianum% of H2ase transcropts C.butyricum
Quantification of mRNA from the hydrogenases of two strains
FISH (Fluorescent In Situ Hybridisation)
Q RT-PCR (Quantitative PCR Real-Time)
0FB
1FB
2FB
4FB
5FB
60.00E+002.00E+084.00E+086.00E+088.00E+081.00E+091.20E+091.40E+091.60E+09
RecA C.butyricumGyrA C.butyricumRecA C.pasteurianumGyrA C.pasteurianum
Techniques:
IV. Molecular ecology of Hydrogen production by Clostridia (COLLABORATION Centre Wallon Biotechnologie Industrielle)