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1                                              R. equi CFS was also examined for the ability to stimula
2                                              R. equi isolates-including MDR ones-were generally susce
3                                              R. equi virulence is dependent on the presence of a larg
4                                              R. equi-stimulated peripheral blood mononuclear cells (P
5                                              R. equi/hoagii, R. corynebacterioides, and R. erythropol
6                       A TRAVAP survey of 215 R. equi strains confirmed the strong link between vapA (
7          In contrast, mice transfused with a R. equi-specific CD4+ Th2 cell line expressed interleuki
8 xamine the mechanism of host defense against R. equi by using a murine model.
9 goal was to passively immunize foals against R. equi by nebulizing mRNA encoding an equine monoclonal
10 ets in the immunoprotective response against R. equi infection.
11                                     Although R. equi infection can produce life-threatening pyogranul
12               We subsequently constructed an R. equi strain lacking only the vapA gene and found that
13 is study, we describe the construction of an R. equi mutant lacking a 7.9 kb DNA region spanning five
14 he taxonomic and nomenclatural issues around R. equi in the light of recent phylogenomic evidence tha
15                             In these assays, R. equi remains fully viable following prolonged exposur
16 ant differences in AST were observed between R. equi and non-equi species.
17        A TLR2 reporter cell was activated by R. equi, and RAW-264 cells transfected with a dominant n
18 e efficient activation of innate immunity by R. equi may account for the relative lack of virulence o
19 m of TLR4 responded normally to infection by R. equi.
20       This "TRAVAP" typing scheme classifies R. equi into 4 categories: traA(+)/vapA(+)B(-), traA(+)/
21 cient to confer virulence to a plasmid-cured R. equi recipient.
22 mid-containing) or avirulent (plasmid-cured) R. equi.
23 face and at the membrane of the host-derived R. equi containing vacuole, thus providing an opportunit
24 te that immunocompetent adult horses develop R. equi-specific CD8+ CTL, which may play a role in immu
25 gns are used as means of controlling endemic R. equi infection on many farms.
26 perimentally infected with Rhodococcus equi (R. equi) and treated with MaR selected for MaR-resistant
27 severity and duration of pneumonia following R. equi infection.
28 ype mice blocked lesion regression following R. equi infection.
29 from soil samples from 100 farms endemic for R. equi infections in Kentucky.
30 in appropriate empiric treatment options for R. equi.
31  polymerase chain reaction typing system for R. equi based on 3 plasmid gene markers: traA from the c
32                       Standard treatment for R. equi disease is dual-antimicrobial therapy with a mac
33 g strains of R. equi (donor) to plasmid-free R. equi strains (recipient) at a high frequency and that
34  and 24 kDa and were recognized by sera from R. equi-infected foals and immune adult horses.
35 coccus equi and specifically to determine if R. equi-specific CD8+ CTL occurred in the blood of immun
36 vel erm(51)-encoding resistance to MLS(B) in R. equi isolates from soil of horse-breeding farms.
37           vapC, -D, and -E are found only in R. equi strains that express VapA and are highly conserv
38 at MaR use promotes multi-drug resistance in R. equi and commensals that are shed into their environm
39 tudy showing a virulence plasmid transfer in R. equi, and it establishes a mechanism by which the vir
40         We show that Himar1 transposition in R. equi is random and needs no apparent consensus sequen
41 rogramming innate immune responses, inducing R. equi-specific adaptive humoral and cell-mediated immu
42 to form peroxynitrite (ONOO(-)), which kills R. equi.
43 p91(phox-/-)) are more susceptible to lethal R. equi infection and display higher bacterial burdens i
44            The role of the surface-localized R. equi lipoprotein VapA (virulence-associated protein A
45  or exposed to soluble R. equi antigen lysed R. equi-infected target cells.
46 two cases suggest the emergence of novel MDR R. equi strains.
47                           Like mycobacteria, R. equi is phagocytosed by alveolar macrophages and repl
48 al growth system was developed for obtaining R. equi CFS antigens.
49 irulence plasmid by an avirulent ancestor of R. equi, coevolution between the plasmid and the chromos
50       We present two HIV-associated cases of R. equi infection from Vietnam and discuss the unique di
51 developed will allow the characterization of R. equi virulence mechanisms and the creation of other a
52 fic CD4+ Th1 cells could effect clearance of R. equi from the lung.
53          Adoptive transfer of a clearance of R. equi from the lungs.
54                       Pulmonary clearance of R. equi requires functional CD4+ T cells and gamma inter
55  sufficient to effect pulmonary clearance of R. equi.
56 uction of the characteristic salmon color of R. equi.
57 nes in neutrophils, higher concentrations of R. equi-specific IgG(1) and IgG(4/7), and a higher numbe
58 ificantly increased tissue concentrations of R. equi.
59 ally replicating plasmid for construction of R. equi mutants.
60 ined that the major virulence determinant of R. equi is the surface bound virulence associated protei
61 ture techniques or serology for diagnosis of R. equi pneumonia in foals.
62 more sensitive and specific for diagnosis of R. equi pneumonia than are other available diagnostic te
63 sociated epidemiologically with emergence of R. equi resistant to MaR.
64 laboratory demonstrated decreased fitness of R. equi strains that were resistant to macrolides, rifam
65     Foals were immunized twice via gavage of R. equi (immunized group) or saline (control group) at a
66 itrite mediates the intracellular killing of R. equi by IFN-gamma-activated macrophages.
67 not necessary for recognition and killing of R. equi-infected cells.
68                                   Killing of R. equi-infected macrophages by effector cells was equal
69 with CTL obtained from the blood, killing of R. equi-infected targets by pulmonary effectors was not
70 regulated in macrophages and in the lungs of R. equi-infected foals, we hypothesized that vapG could
71  presence of VapA inhibits the maturation of R. equi-containing phagosomes and promotes intracellular
72 ts the predominantly opportunistic nature of R. equi infection in this host and a zoonotic origin.
73 hat recognized the vapA virulence plasmid of R. equi had a diagnostic sensitivity of 100% and specifi
74 uld be extremely useful in the prevention of R. equi disease in horses.
75 n resistance on intracellular replication of R. equi in equine pulmonary macrophages and in an in viv
76                                    The SD of R. equi, Nocardia sp., M. nonchromogenicum, M. monacense
77 gens and reduce the duration and severity of R. equi pneumonia.
78 ansferred from plasmid-containing strains of R. equi (donor) to plasmid-free R. equi strains (recipie
79                          Virulent strains of R. equi bear a large plasmid that is required for intrac
80                               All strains of R. equi isolated from foals and approximately a third is
81  and between traA(+)/vapAB(-)--a new type of R. equi plasmid--and cattle.
82   Progress in the molecular understanding of R. equi and its recent rise as a novel paradigm of multi
83 proof of a role for vapA in the virulence of R. equi, and demonstrate that its presence is essential
84  Inflammatory cells from either L. major- or R. equi-infected C57BL/6 mice were sensitive to TNF-indu
85              Best known as a horse pathogen, R. equi is commonly isolated from other animal species,
86                  The standard for preventing R. equi pneumonia in foals is transfusion of hyperimmune
87                       Loss of pVAPN rendered R. equi avirulent in macrophages and mice.
88 ction of susceptible and macrolide-resistant R. equi strains from equine clinical cases using a panel
89  treated with MaR selected for MaR-resistant R. equi, whereas MaR-susceptible R. equi out-competed re
90 cidence of macrolide- and rifampin-resistant R. equi isolates has been documented.
91                As typical in the rhodococci, R. equi niche specialization is extrachromosomally deter
92 e two proteins are not expressed by the same R. equi isolate.
93  infected with R. equi or exposed to soluble R. equi antigen lysed R. equi-infected target cells.
94 R-resistant R. equi, whereas MaR-susceptible R. equi out-competed resistant isolates in GaM-treated o
95  the absence of antibiotics, the susceptible R. equi isolate outcompeted the macrolide- or rifampin-r
96 mmune adult horses and provide evidence that R. equi CFS proteins are antigen targets in the immunopr
97           In this study, the hypothesis that R. equi-specific cytotoxic T lymphocytes (CTL) are prese
98  and VapE, which are encoded by genes on the R. equi virulence plasmid.
99 nd alveolar macrophages, suggesting that the R. equi-specific, major histocompatibility complex-unres
100 are with 10 cases diagnosed (majority due to R. equi) and managed.
101 ur data indicate that early life exposure to R. equi in the gastrointestinal tract can modulate innat
102 8+ CTL, which may play a role in immunity to R. equi.
103 antly more favorable AST profile relative to R. equi.
104 rophages were fully capable of responding to R. equi infection, and because RAW-264 cells transfected
105 oduced virtually no cytokines in response to R. equi infection, implicating a TLR pathway.
106 N-gamma producing lymphocytes in response to R. equi stimulation indicating T helper type 1 response
107 e exhibited diminished cytokine responses to R. equi.
108 bited markedly reduced cytokine responses to R. equi.
109 iotics are the standard of care for treating R. equi pneumonia in foals, and adjunctive therapies are
110 macrophage replication defect of a wild type R. equi strain lacking the vapA gene and enhances the pe
111                             Unlike wild-type R. equi which replicates intracellularly, both of the mu
112 tudies showed that, in contrast to wild-type R. equi, the riboflavin-requiring mutant is attenuated b
113 h equine (pVAPA) and porcine (pVAPB variant) R. equi isolates.
114 cteria to ONOO(-) efficiently kills virulent R. equi.
115 e adult horses were challenged with virulent R. equi, and cells from the bronchoalveolar lavage fluid
116 r ability to clear a challenge with virulent R. equi.
117 e with VapA; the proteins are expressed when R. equi is cultured at 37 degrees C but not at 30 degree
118 ose of this study was to investigate whether R. equi-specific CD4+ Th1 cells could effect clearance o
119        Our findings support a model in which R. equi virulence is conferred by host-adapted plasmids.
120 al foals after intrabronchial challenge with R. equi.
121 equi isolated from young horses (foals) with R. equi pneumonia, carry an 80-90 kb virulence plasmid a
122 ntigen-presenting cells either infected with R. equi or exposed to soluble R. equi antigen lysed R. e
123 lar macrophages after ex vivo infection with R. equi.
124  foals were challenged intrabronchially with R. equi.
125  stimulation of pulmonary T-lymphocytes with R. equi CFS resulted in significant proliferation and a
126 ek after experimental infection of mice with R. equi resulted in more severe disease and significantl
127 ived pulmonary T lymphocytes stimulated with R. equi lysed infected alveolar macrophages and peripher

 
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