Real-time PCR was used to detect and quantify Mycobacterium bovis cells in

naturally infected soil and badger faeces. Immunomagnetic capture,

immunofluorescence and selective culture confirmed species identification and cell

viability. These techniques will prove useful for monitoring M. bovis in the

environment and for elucidating transmission routes between wildlife and cattle

Sweeney, F. P.

Courtenay, Orin

Hibberd, V.

Hewinson, R. G.

Reilly, L. A.

Gaze, William H.

Wellington, E. M. H.

English

PubMed

summary:This paper analyzes the BIBO stability of fractional exponential delay systems which are of retarded or neutral type. Conditions ensuring stability are given first. As is the case for the classical class of delay systems these conditions can be expressed in terms of the location of the poles of the system. Then, in view of constructing robust BIBO stabilizing controllers, explicit expressions of coprime and Bézout factors of these systems are determined. Moreover, nuclearity is analyzed in a particular case

Bonnet, Catherine

Partington, Jonathan R.

Institute of Mathematics AS CR, v. v. i.

Stabilization of fractional exponential systems including delays

Crossref

The authors consider in this paper the simultaneous problem of optimal robust stabilization and optimal tracking for single-input/single-output (SISO) systems in an L-∞-setting using a two-parameter compensator scheme. Optimal robustness is linked to the work done by Georgiou and Smith in the L-2-setting. Optimal tracking involves the resolution of L-1-optimization problems. The authors consider in particular the robust control of delay systems. They determine explicit expressions of the Bezout factors for general delay systems which are in the Callier-Desoer class β(0). Finally, they solve several general L-1-optimization problems and give an algorithm to solve the optimal robust control problem for a large class of delay systems

Bonnet, C.

Partington, J.R.

White Rose Research Online

Bezout factors and L-1-optimal controllers for delay systems using a two-parameter compensator scheme

Czech digital mathematics library

Warwick Research Archives Portal Repository

 University of Warwick institutional repository: http://go.warwick.ac.uk/wrap  This paper is made available online in accordance with publisher policies. Please scroll down to view the document itself. Please refer to the repository record for this item and our policy information available from the repository home page for further information.  To see the final version of this paper please visit the publisher’s website. Access to the published version may require a subscription. Author(s):  F.P.Sweeney, O. Courtenay, V. Hibberd, R.G. Hewinson, L.A. Reilly , W.H.Gaze and E.M.H. Wellington Article Title:  Environmental monitoring of Mycobacterium bovis in badger feces and badger sett soil by real-time PCR, as confirmed by immunofluorescence, immunocapture, and cultivation Year of publication: 2007 Link to published article: http://dx.doi.org/10.1128/AEM.00978-07 Publisher statement:  Copyright © 2007, American Society for Microbiology and/or the Listed Authors/Institutions. All Rights Reserved.     Environmental monitoring of Mycobacterium bovis in badger faeces and badger 1 sett soil using real-time PCR, confirmed by immunofluorescence, 2 immunocapture and cultivation. 3  4 Running title: Real-time PCR of environmental Mycobacterium bovis 5  6 F.P.Sweeney1*, O. Courtenay2, V. Hibberd1, R.G. Hewinson3, L.A. Reilly2, W.H. 7 Gaze1 and E.M.H. Wellington1. 8  9 1Microbiology Group and 2Ecology & Epidemiology Group, Department of 10 Biological Sciences, University of Warwick, Coventry, CV4 7AL, UK. 11 3Veterinary Laboratories Agency, New Haw, Addlestone, Surrey, KT15 3NB, UK. 12  13 *Tel: +44 (0)2476 522431 14  Fax: +44 (0)2476 523701 15 Email: f.p.sweeney@warwick.ac.uk 16  17 ACCEPTED Copyright © 2007, American Society for Microbiology and/or the Listed Authors/Institutions. All Rights Reserved.Appl. Environ. Microbiol. doi:10.1128/AEM.00978-07 AEM Accepts, published online ahead of print on 28 September 2007Abstract  18 Real-time PCR was used to detect and quantify Mycobacterium bovis cells in 19 naturally infected soil and badger faeces. Immunomagnetic capture, 20 immunofluorescence and selective culture confirmed species identification and cell 21 viability. These techniques will prove useful for monitoring M. bovis in the 22 environment and for elucidating transmission routes between wildlife and cattle.  23  24  25 Previous studies of Mycobacterium bovis shed into the environment by infected hosts 26 using conventional PCR with primers targeting the MPB70 antigen gene (specific to 27 the M. tuberculosis complex) provided evidence that the organism is likely to persist 28 in the environment for at least 15 months post removal of the known animal reservoirs 29 (16), and that the probability of detection of M. bovis in soil and badger faeces is 30 correlated with the prevalence of excreting badgers (2). For the purpose of 31 epidemiological studies, M. bovis detection techniques must be 100% species specific 32 with robust and reliable quantification. 33  34 Real time PCR has advantages over conventional PCR because it allows absolute 35 quantification by comparison to a standard curve of known target sequence numbers. 36 The complete genome sequence of M. bovis (5) has been used to design primers 37 flanking a region of difference (RD4) between the sequence of M. bovis DNA and that 38 of other M. tuberculosis complex members (1). The presence of M. bovis is confirmed 39 using a fluorescent (TaqMan) probe which discriminates M. bovis from other 40 Mycobacterium tuberculosis complex members since it hybridises with both the 5’ 41 ACCEPTEDand the 3’ RD4 deletion flanking sequences which only occur directly adjacent to 42 each other in M. bovis (1).  43  44 M. bovis cannot be directly cultured from soil due to the harsh decontamination 45 techniques required to remove competing organisms. This limitation was overcome in 46 a previous study by using immunomagnetic capture (IMC) to extract cells of M. bovis 47 from mixed cell communities using a poly-clonal antibody to M. bovis BCG, and thus 48 enabling cultivation of M. bovis from soil samples for the first time (13). Greater 49 specificity could be achieved using a monoclonal antibody, MBS43 (14, 15), which 50 recognises MPB83, a glycosylated cell wall associated protein (8), differentiating M. 51 bovis from other members of the M. tuberculosis complex (6).  52  53 We report here the first use of an M. bovis-specific real-time PCR to detect and 54 quantify M. bovis DNA in environmental samples, and confirm the presence of viable 55 cells of M. bovis using IMC, immunofluorescence and cultivation.  56  57 Badgers are an important wildlife reservoir of M. bovis in the UK, and infected 58 badgers can excrete the organism into the environment (4, 13). Social groups of 59 badgers dig underground tunnel systems known as setts and they defecate into 60 communal “latrines”, which are often located on cattle pasture. Soil was collected 61 from 7 badger setts and faeces collected from 5 badger latrines during September 62 2006 on two cattle farms in a region of the UK endemic for bovine tuberculosis (bTB). 63 Replicate samples were taken from within 10m of each other at any one sett or latrine, 64 though the setts and latrines were variable in size. The average distance between 65 nearest neighbour sampled setts was 195m (range 40m-380m), and 234m (range 60m-66 ACEPTED400m) between nearest neighbour sampled latrines. The study farms were not under 67 bTB restriction at the time of sampling, but had experienced tuberculin skin test 68 positive heard breakdowns, as defined by Defra, in the past. These sites were chosen 69 as they had previously tested positive for M. bovis using conventional PCR (2). Four 70 soil samples were used as negative controls: two from an area non-endemic for bTB 71 and two endemic samples that had tested negative for M. bovis using the MPB70 PCR 72 (16). Total community DNA was extracted from 0.2g of each sample using Qiagen 73 Stool DNA extraction kit (Qiagen UK) following the manufactures instructions. 74 Triplicate reactions were carried out for all environmental samples, standards and no 75 template controls using real-time PCR. For each reaction, the total reaction volume 76 was 25 µl comprising 12.5 µl TaqMan universal PCR master mix, 1 µl (20 pmol ) 77 forward RD4 flanking primer (5’ TGTGAATTCATACAAGCCGTAGTCg 3’), 1 µl 78 (20 pmol) reverse RD4 flanking primer (5’ CCCGTAGCGTTACTGAGAAATTGC 79 3’) and 1 µl (20 pmol) of the Probe ( 5’ FAM-80 AGCGCAACACTCTTGGAGTGGCCTAC 3’- TAMRA), 2.5 µl of a 10 mg/ml BSA 81 solution 6 µl nuclease free sterile water and 1 µl of a 1:10 dilution of the total 82 community DNA.   83  84 IMC was carried out as previously described (13), but with duplicate 0.5g aliquots of 85 the environmental samples blocked with 3% BSA in PBS overnight at 4oC. Dynal 86 magnetic beads (Invitrogen UK) 50µl (50mg) pre-coated with goat anti-mouse 87 antibody were linked to 100 µg MBS43. The reaction was incubated for 3 h with 88 shaking at 4oC. The antibody coated beads were then added to the blocked 89 environmental sample and incubated for 3 h at 4oC with shaking. Cells of M. bovis 90 were captured and separated using a magnetic device (Dynal UK), separated cells 91 ACETEDwere washed three times with PBS containing 0.1% nonident and resuspended in 92 200µl of PBS. M. bovis was cultivated on non-acidified pyruvate LJ media slopes 93 (Media for Mycobacteria Ltd., Cardiff, UK) incubated at 37oC for 4 weeks. Single 94 colonies were transferred to Kirchner medium (Media for Mycobacteria Ltd.), 95 supplemented with sodium pyruvate (4 g / litre) and the following antibiotics, 96 Polymyxin B (200 000 units/ litre), Ticarcillin (100 mg / litre), Trimethoprim (10 mg / 97 litre) and  the anti fungal amphotericin B (10mg / litre). A commercially labelled 98 polyclonal antibody to M. bovis BCG (DAKO) was coupled to FITC labelled goat 99 anti-rabbit IgG by incubating 50 µg of each at 4oC with shaking. 10 µl was added to 100 50 µl of the immunocaptured cells. DAPI was also added and the solution left for 1 h 101 at 4oC. Cells were fixed with 4% glutaraldehyde for 2 h before fluorescence 102 microscopy.  103  104 TaqMan real-time PCR detected the presence of M. bovis in all 12 samples from 105 infected setts and latrines, but no M. bovis DNA was amplified from the four negative 106 controls. Gene copies per gram of sample ranged from 6.8x104 to 5.4x106 (Fig 1), 107 with quantities appearing more variable between sett samples than between latrine 108 samples, although the mean cell count did not differ significantly between sett and 109 latrine samples (F1,10=0.77, NS), nor was there a significant difference in the cell 110 count variances between sample types (Bartlett’s χ2=2.01, P=0.156). The product was 111 confirmed as M. bovis by its size (142 bp) and sequence. 112  113 ACEPTED110100100010000100000100000010000000L1 L2 L3 L4 L5 S1 S2 S3 S4 S5 S6 S7SampleGenome equivalent per gram of sample 114 Figure 1. The mean number of M. bovis cell copies per gram of environmental 115 sample (L = latrine; S = sett) estimated by Taq Man real-time PCR. Error bars 116 represent the 95% confidence intervals around the mean counts from three replicates 117 per sample.  118  119 Immunomagnetic capture was performed on all of the positive samples and in all 120 cases confirmed the presence of M. bovis cells by subsequent cultivation. M. bovis 121 cells from one sample (L3) captured by the MBS43 coated magnetic beads and 122 stained with FITC coupled M. bovis BCG antibody are shown in Fig. 2. DAPI stain 123 detected the captured bacteria and FITC fluorescence was seen to co-localise with the 124 cells. 125  126 ACCEPTED 127 Figure 2. Immunocaptured M. bovis attached to magnetic particles stained with DAPI 128 (blue) and FITC (green). 600X oil immersion. 129  130 Captured cells from all of the 12 samples were inoculated onto LJ media slopes 131 (Media for Mycobacteria Ltd., Cardiff, UK) which gave colonies after 4 weeks at 132 37oC. These were sub-cultured into Kirchner medium (supplemented with 4 g/l w/v 133 Na pyruvate and BSA (Media for Mycobacteria Ltd., Cardiff, UK). 134  135 Many pathogenic bacteria can survive in the environment (7), and several members of 136 the Mycobacterium genus are known to persist even under extremely hostile 137 conditions (12). Several properties that are common to all mycobacteria may help M. 138 bovis endure extreme environmental conditions following excretion by an infected 139 host, and a reservoir of the organism in the environment could potentially be a source 140 of infection to cattle and other susceptible species. Bovine tuberculosis is an endemic 141 disease in badgers in Great Britain and Ireland (9), however the route or routes of 142 ACCEPTEDtransmission to cattle are poorly understood. Cattle are known to be highly susceptible 143 to aerosol transmission (11) but can also become infected through ingestion, although 144 experiments have shown that as many as 107 bacilli must be ingested to cause 145 infection by this route (3, 10). Gallagher and Clifton-Hadley (4) estimated by 146 selective cultivation the number of M.bovis bacilli that badgers with advanced 147 milliary disease can shed into the environment. They cultivated 200 x 103 and 68 c.f.u. 148 per g from two separate clinical faecal samples and 217 x 103 and 250 x 103 c.f.u. per 149 ml from two separate urine samples (4). The results of this study using real time PCR 150 show cell densities of 6.8 x 104 to 5.4 x 106 M. bovis cells per gram of soil at badger 151 setts and of faeces at badger latrines, which we assume to be typical in this infected 152 badger population. Previous estimates of cell numbers in similar samples were 153 between 2.8 x 105 and 3.2 x 105 using a different method (MPB70 and Rv1510 154 primers with PCR product quantified by pixel intensity) (13). In the current study 155 there was no statistical difference between the mean and variance of cell counts at 156 setts vs. latrines, however, on visual inspection the quantities detected at setts 157 appeared to be more variable than those at latrines. If this proves to be the case, it may 158 be due to the greater variability in the distribution of micro-organisms in soil 159 compared to faeces, and/or differences in the excretory behaviour of badgers at setts 160 compared to at latrines. 161  162 In conclusion, we have developed an M. bovis specific molecular detection technique, 163 based on real-time PCR, for monitoring and quantifying cells in environmental 164 samples. This method will be useful for identifying sites of contamination on farms 165 that may constitute an infection risk to cattle and wildlife.  166  167 ACCEPTEDThe work was conducted with financial support from the BBSRC (grant 168 BBS/B/08868 awarded to O.C. and E.M.W). The authors wish to thank the farmers 169 for granting permission to take samples.  170  171 References  172  173 1. Brosch R., S.V. Gordon, M. Marmiesse, P. Brodin, C. Buchrieser, K. 174 Eiglmeier, T. Garnier, C. Gutierrez, R.G. Hewinson, K. Kremer, L. M. 175 Parsons, A. S. Pym, S. Samper, D. van Soolingen, and S. T. Cole. 2002. A new 176 evolutionary scenario for the Mycobacterium tuberculosis complex. PNAS 177 99:3684-3689. 178  179 2. Courtenay, O., L.A. Reilly, F.P. Sweeney, V. Hibberd, S. Bryan, A. Ul-Hassan,     180 C. Newman, D.W. Macdonald, R.J. Delahay, G.J. Wilson and E.M.H. 181 Wellington.  2006. Is Mycobacterium bovis in the environment important for the 182 persistence of bovine tuberculosis? Biol. Lett. 2:460-462. 183  184 3. Francis, J. 1947. Bovine tuberculosis: including a contrast with human 185 tuberculosis, Staples Press, London, p92. 186  187 4. Gallagher, J. and R.S. Clifton-Hadley. 2000. Tuberculosis in badgers: a review 188 of the disease and its significance for other animals.  Res. Vet. Sci. 69:203-217. 189  190 5. Garnier, T., K. Eiglmeier, J.C. Camus, N. Medina, H. Mansoor, M. Pryor, S. 191 Duthoy, S. Grondin, C. Lacroix, C. Monsempe, S. Simon, B. Harris, R. Atkin, 192 ACCEPTEDJ. Doggett, R. Mayes, L. Keating, P.R. Wheeler, J. Parkhill, B.G. Barrell, S.T. 193 Cole, S.V. Gordon and R.G. Hewinson. 2005. The complete DNA sequence of 194 Mycobacterium bovis. PNAS 45:1113-1244. 195  196 6. Goodger J., A. Nolan, W.P. Russell, D.J. Dalley, C.J. Thorns, F.A. Stuart, P. 197 Croston and D.G. Newell. 1994. Serodiagnosis of Mycobacterium bovis infection 198 in badgers: development of an indirect ELISA using a 25 kDa antigen. Vet. Rec. 199 135:82-85.   200  201 7. Guan, T.Y. and R.A. Holley. 2003. Pathogen survival in swine manure 202 environments and transmission of human enteric illness – a review. J. Environ. 203 Qual. 32:383-392. 204  205 8. Hewinson, R.G., S.L. Michell, W.P. Russell, R.A. McAdam and W.R. Jacobs 206 Jr. 1996. Molecular characterisation of MPT83: a seroactive antigen of 207 Mycobacterium tuberculosis with homology to MPT70. Scand. J. Immunol. 208 43:490-499. 209  210 9. Nolan, A. and J.W. Wilesmith. 1994. Tuberculosis in badgers (Meles meles). Vet. 211 Microbiol. 28:103-109. 212  213 10. O’Reilly, L.M. and C.J. Daborn. 1995. The epidemiology of Mycobacterium 214 bovis infections in animals and man: a review. Tuber. Lung Dis. 76 (S1):1-46. 215  216 ACCEPTED11. Palmer, M.V., W.R. Waters and D.L. Whipple. 2003. Aerosol exposure of 217 virulent Mycobacterium bovis to cattle. Tuberculosis 82:275-282. 218  219 12. Primm, T.P., C.A. Lucero and J.O. Falkinham 3rd. 2004. Health impacts of 220 environmental mycobacteria. Clin. Microbiol. Rev. 17:98-106. 221  222 13. Sweeney, F.P., O. Courtenay, A. Ul-Hassan, V. Hibberd, L.A. Reilly and 223 E.M.H. Wellington. 2006. Immunomagnetic recovery of Mycobacterium bovis 224 from naturally infected environmental samples. Lett. Appl. Microbiol. 2:460-462. 225  226 14. Wiker, H.G., S. Nagai, R.G. Hewinson, W.P. Russell and M. Harboe. 1996. 227 Heterogenous expression of the related MPB70 and MPB83 proteins distinguish 228 various substrains of Mycobacterium bovis BCG and Mycobacterium tuberculosis 229 H37Rv. Scand. J. Immunol. 43:374-80. 230  231 15. Wiker, H.G., K.P. Lyashchenko, A.M. Aksoy, K.A. Lightbody, J.M. Pollock, 232 S.V. Komissarenko, S.O. Bobrovnik, I.N. Kolesnikova, L.O. Mykhalsky, M.L. 233 Gennaro and M. Harboe. 1998. Immunochemical characterization of the 234 MPB70/80 and MPB83 proteins of Mycobacterium bovis. Infect. Immun. 235 66:1445-52. 236  237 16. Young, J.S., E. Gormley and E.M.H. Wellington. 2005. Molecular detection of 238 Mycobacterium bovis and Mycobacterium bovis BCG (Pasteur) in soil. Appl. 239 Environ. Microbiol 71:1946-1952 240 ACCE TED