Applied and Environmental Microbiology, May 2004, p . 3180-3182, Vol . 70, No . 5

Specific PCR Assay for a Tannin-Tolerant Selenomonas ruminantium Isolate, Derived from Helicase Coding Sequences

Richard Bishop,^* Moses Obura, David Odongo, and Agnes Odenyo

The International Livestock Research Institute, Nairobi, Kenya, and Addis Ababa, Ethiopia

Received 21 January 2004/ Accepted 28 January 2004

 
The nucleotide sequences of the two EAT2-specific sequences and of a third clone that hybridized more strongly to EAT2 than to other isolates were determined . Blast X searches of the NCBI databases revealed that clones 1 (524 bp) and 3 (941 bp) contained open reading frames (ORFs) with significant amino acid identity to different mobile element or prophage-encoded ORFs . For clone 1 there was very high identity to a superfamily II RNA/DNA helicase gene of Lactobacillus gasseri (accession no . ZP_00046684) and a phage-associate helicase of Streptococcus pyogenes (1) (NP_665244) . These corresponded to 72% identity over 123 amino acids (aa) and 56% identity over 122 aa, respectively (E values: 2e-47 and 1e-33) . The most significant match of clone 3 was with a transposase of Fusobacterium nucleatum (5) (NP_602338), corresponding to 38% identity over 270 aa (4e-42) . Prophages have been described previously from rumen bacteria, including S . ruminantium (6) . Our data indicate that coding sequences within prophages can have a wide phylogenetic distribution among different genera but can also be quite restricted among isolates within a single species . The sequence of clone 2 (722 bp) exhibited identity with ORFs of human endosymbionts, the highest identity being to a conserved hypothetical protein of Bacteroides thetaiotaomicron (13) (NP_809516) .

To investigate the potential of these sequences for monitoring bacteria introduced into the rumen, PCR primers for amplification of approximately 200 bp from clones 1 and 2 were designed by using Primer3 software (http://frodo.wi.mit.edu/) . The sequence 1 primers were (5' TCACTTGGAGCCTGGAACTT 3') and (5' TCATTTCTGCTCCCCTCCTA 3') . Sequence 2 primers were (5' GGTACAAAAGCTGGGCATGT 3') and (5' GTCAGCCTGCCTGGTATCAT 3') . These primers were applied to DNA (50 ng) from seven S . ruminantium isolates (10) in a standard PCR by using Taq polymerase (Promega) in the manufacturer's buffer under the following parameters: 1 min at 94°C, 1 min at 55°C, and 1 min at 72°C for 30 cycles, followed by a 5-min extension at 72°C . Both sets of primers generated products only from EAT2 DNA . Representative results are shown for the PCR primers derived from clone 1 in Fig . 1B . The primers were also applied to total DNA that had been prepared from the gastrointestinal contents of wild and domestic ungulates by a physical disruption method with zirconia silicon beads and a bead beater (11), collected as described previously (8, 9, 10) . Neither set of primers generated any products from 300 ng of total DNA prepared from 10 µl of rumen fluid from five different Bos indicus cattle . However, a product was generated from EAT2 genomic DNA mixed with 300 ng of rumen fluid DNA . Representative results from using the clone 1 primers are shown in Fig . 2A . A similar PCR was performed by using total gastrointestinal fluid DNA from one sheep, one goat, and six wildife species, Thompson's (Gazella thompsoni) and Grant's (Gazella granti) gazelles, eland (Taurotragus oryx), impala (Aepyceros melampus), Coke's hartebeest (Alcephalus busephalus), and one nonruminant, i.e., zebra (Equus burchelli) . No products were generated from these samples . To evaluate the sensitivity of detection by PCR, decreasing quantities of serially diluted EAT2 DNA were combined with 300 ng of total rumen fluid DNA from cattle and were amplified with the primers derived from clone 1 . It was possible to detect 10 pg of EAT2 DNA under these conditions (Fig . 2B, lane 5) . Approximately 2,000 to 5000 genome equivalents of S . ruminantium (assuming a genome size of 2 to 5 megabases) could be detected against a background of total DNA generated from approximately 10⁸ bacteria, indicating the potential utility of the probe for tracking EAT2 introduced into domestic ruminants .

 
Our results confirm the effectiveness and ease of application of the SSH technique (2) for isolating sequences differing between bacterial isolates within a species, relative to earlier subtractive methods . The data also suggest that the technique may selectively result in isolation of coding sequences . The 16S ribosomal DNA sequences of the S . ruminantium isolates used in this study were 99% identical, and they clustered closely in dendrograms derived from genome-wide amplified fragment length polymorphism analysis (10) .

This is ILRI publication number 200374 .

Present address: The International Centre for Research on Agroforestry, Nairobi, Kenya .

1. Beres, S . B., G . L . Sylva, K . D . Barbian, B . Lei, J . S . Hoff, N . D . Mammarella, M . Y . Liu, J . C . Smoot, S . F . Porcella, L . D . Parkins, D . S . Campbell, T . M . Smith, J . K . McCormick, D . Y . M . Leung, P . M . Schlievert, and J . M . Musser. 2002 . Genome sequence of a serotype M3 strain of a group A Streptococcus: phage-encoded toxins, the high-virulence phenotype, and clone emergence . Proc . Natl . Acad . Sci . USA 99:10078-10083.
2. Diatchenko, L., Y . F . Lau, A . P . Campbell, A . Chenchik, F . Moqadam, B . Huang, S . Lukyanov, K . Lukyanov, N . Gurskaya, E . D . Sverdlov, and P . D . Siebert. 1996 . Suppression subtractive hybridization: a method for generating differentially regulated or tissue-specific cDNA probes and libraries . Proc . Natl . Acad . Sci . USA 93:6025-6030.
3. Gursakya, N . G., L . Diatchenko, A . Chenchik, P . D . Siebert, G . L . Khaspekov, K . A . Lukyanov, L . L . Vagner, O . D . Ermolaeva, A . Lukyanov, and E . D . Sverdlov. 1996 . Equalizing cDNA subtraction based on selective suppression of polymerase chain reaction: cloning of Jurkat cell transcripts induced by phytohemagglutinin and phorbol 12-myristate 13-acetate . Anal . Biochem . 240:90-97.
4. Hagerman, A . E., C . T . Robbins, Y . M . Weerasuriya, T . C . Wilson, and C . McArthur. 1992 . Tannin chemistry in relation to digestion . J . Range Manag . 45:57-62.
5. Kapatral, V., I . Anderson, N . Ivanona, G . Reznik, T . Los, A . Lykidis, A . Bhattacharyya, A . Bartman, W . Gardner, G . Grechkin, L . Zhu, O . Vasieva, L . Chu, Y . Kogan, O . Chaga, E . Goltsman, A . Bernal, N . Larsen, M . D'Souza, T . Walunas, G . Pusch, R . Haselkorn, M . Fonstein, N . Kyrpides, and R . Overbeek. 2002 . Genome sequence and analysis of the oral bacterium Fusobacterium nucleatum strain ATCC 25586 . J . Bacteriol . 184:2005-2018.
6. Lockington, R . A., G . E . Attwood, and J . D . Brooker. 1988 . Isolation and characterization of a temperate bacteriophage from the ruminal anaerobe Selenomonas ruminantium . Appl . Environ . Microbiol . 54:1575-1580.
7. Nelson, K . E., M . L . Thonney, T . K . Woolston, S . H . Zinder, and A . N . Pell. 1998 . Phenotypic and phylogenetic characterization of ruminal tannin-tolerant bacteria . Appl . Environ . Microbiol . 64:2824-3830.
8. Nelson, K . E., S . Zinder, I . Hance, P . Burr, D . Odongo, D . Wasawo, A . Odenyo, and R . Bishop. 2003 . Phylogenetic analysis of gastrointestinal tract microbial populations in the wild herbivore gastrointestinal tract: insights into an unexplored niche . Environ . Microbiol . 5:1212-1220.
9. Odenyo, A . A., and P . O . Osuji. 1998 . Tannin-tolerant ruminal bacteria from East African ruminants . Can . J . Microbiol . 44:905-909.
10. Odenyo, A . A., R . Bishop, G . Asefa, R . Jamnadass, D . Odongo, and P . Osuji. 2001 . Characterisation of tannin-tolerant bacterial isolates from East African ruminants . Anaerobe 7:5-15.
11. Reilly, K., and G . T . Attwood. 1998 . Detection of Clostridium proteoclastum and closely related strains in the rumen by competitive PCR . Appl . Environ . Microbiol . 64:907-913.
12. Skene, I . K., and J . D . Brooker. 1995 . Characterisation of tannin acylhydrolase activity in the ruminal bacterium Selenomonas ruminantium . Anaerobe 1:321-327.
13. Xu, J., M . K . Bjursell, J . Himrod, S . Deng, S . K . Carmichael, H . C . Chiang, L . V . Hooper, and J . I . Gordon. 2003 . A genomic view of the human-Bacteroides thetaiotaomicron symbiosis . Science 299:2074-2076.

Free Online Full-text Article

What Is Bioremediation?, What Is Anthrax?, What Is Staphylococcus Aureus?, What Is Functional Genomics?, What Is Biotechnology?, n, Microorganisms, c, Microbiology, r, Bacterium, n, Bacteria, r, Microorganism, a, Erythromycin, i, Bactericidal, c, Antimicrobials, a, Escherichia coli, r, Lactococci, o, Streptococci, c, Streptococcal, r, Salmonella, n, Bacteria, s, Bacillus subtilis, a, Clostridia, o, S. cerevisiae, e, Campylobacter, e, Salmonella typhimurium, i, Bacillus, n, Candida albicans, n, Staphylococcus aureus, s, Bactericidal, s, Enterococci, e, Beta lactamase, c, Vancomycin




 

© 2005 Transgalactic Ltd (manufacturer of Bioscreen C software) | Privacy Statement | P.O. Box 1393, 00101 Helsinki, Finland, phone: +358 9 85172920, fax: +358 9 8749481, e-mail: microbiology@bionewsonline.com
 

Last modified: May 25, 2005