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Query: UMLS:C0026918 (
Mycobacterium
)
52,428
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
Tumor necrosis factor, lymphocyte-activating factor, and enhanced levels of type I interferon were found in serum samples taken 2 h after mice infected with Plasmodium vinckei subsp. petteri received a small intravenous injection of endotoxin. These three mediators are among those released when mice receive an endotoxin injection 2 weeks after
Mycobacterium
bovis BCG or Corynebacterium parvum have been administered. There is indirect evidence that this wider range of mediators is also released in P. vinckei subsp. petteri-infected mice given parenteral endotoxin. A recent report that endotoxin is detectable in the plasma of malaria-infected mice and children implies that these mediators may also be released in the acute phase of the natural infection. We propose that these macrophage-derived mediators may be important in the glucocorticoid antagonism, bone marrow depression, fever, hypergammaglobulinemia, splenomegaly, elevation of
serum amyloid A
, consumptive coagulopathy, and shock syndrome with associated organ damage which can accompany malaria. The intraerythrocytic parasite death seen at crisis in some malarias, as well as the subsequent development of specific protective immunity, may also depend on these mediators.
...
PMID:Possible importance of macrophage-derived mediators in acute malaria. 616 64
Sixteen out of 45 (36%) leprosy patients with clinical features of acute erythema nodosum leprosum (ENL) did not show the characteristic presence of neutrophils (polymorphs) in histology of the ENL lesion. The acute-phase reactants,
serum amyloid A
(
SAA
) and C-reactive protein (CRP) which are systemic markers of inflammation, and IgM and IgG antibody to
Mycobacterium
leprae were determined in these patients in order to understand the differences in histological diagnosis. Both
SAA
and CRP were elevated in ENL patients, irrespective of the presence of polymorph infiltrates, as compared to nonreactional lepromatous patients, patients with histologically confirmed reversal reactions and endemic controls, indicating that all clinically diagnosed ENL patients had ongoing inflammatory reactions. On the other hand, IgM and IgG antibodies were significantly lower (> 70%) in ENL patients as compared to nonreactional lepromatous patients. When the two ENL groups [ENL-PMN+ve (positive for neutrophils) and ENL-PMN-ve (negative for neutrophils)] were compared, there were no significant differences in the mean
SAA
, IgM or IgG antibody concentrations, but CRP was eightfold lower in ENL-PMN-ve as compared to the ENL-PMN+ve group. This may indicate that the timing or modulation of the reaction was different in the two ENL groups. Thus, measurement of the acute-phase response and the ratio of
SAA
/CRP in particular are helpful in the clinical diagnosis of ENL reactions in leprosy.
...
PMID:Clinical and histological discrepancies in diagnosis of ENL reactions classified by assessment of acute phase proteins SAA and CRP. 760 17
The localization of amyloid fibril components and the cells related to the formation and resorption of the fibrils are still controversial. We conducted a time-kinetic study to analyse the process of amyloid fibril deposition in the spleen of an AA amyloidosis animal model immunohistochemically. Murine AA amyloidosis was induced by an emulsion injection composed of Freund's complete adjuvant and
Mycobacterium
butyricum. The
serum amyloid A
level was the highest at 3 days after the induction and gradually decreased. The amyloid deposition was first detected in extracellular spaces in the marginal zone of the spleen at 7 days after induction. F4/80 positive red pulp macrophages increased in number after the induction and accumulated near the amyloid deposition areas. Amyloid P component (APC) and chondroitin sulphate proteoglycan (CSPG), which are composed of amyloid fibril, were detected in the cytoplasm of F4/80 positive red pulp macrophages and ER-TR9 positive marginal zone macrophages, respectively, then localized in the amyloid deposition areas. APC was also localized in CSPG positive and F4/80 negative cells, which might be fibroblasts at 3 days. These results suggest a close association of APC positive/ER-TR9 positive macrophages and APC positive/CSPG positive fibroblasts in the formation of amyloid fibrils and F4/80 positive macrophages with the resorption of fibrils.
...
PMID:Histological study of experimental murine AA amyloidosis. 1459 3
Haem oxygenase (HO)-1, a rate-limiting enzyme in the degradation of haem, is increased in Alzheimer's disease and in inflammations such as AA amyloidosis. However, the specific association of HO-1 is poorly understood in AA amyloidosis. In this study, we designed the experiment to reveal the contribution and association of HO-1 in the spleen during experimental murine AA amyloidosis. Experimental murine AA amyloidosis was induced with injection of an emulsion consisting of Freund's complete adjuvant and
Mycobacterium
butyricum. The
serum amyloid A
level was highest on day 3. The distribution of cells containing iron, indicating an increase of HO-1 in the red pulp, was detected with Berlin blue staining. AA amyloid formation was immunohistochemically detected as a marker by chondroitin sulphate proteoglycan (CSPG), one of the components of AA amyloid fibrils. Immunolocalizations of HO-1 and CSPG indicated a conspicuous increase and scattering of positive cells in the red pulp of the spleen. Double positive cells were not detected. On day 7, amyloid deposition was detected with Congo red staining in the extracellular spaces in the marginal zone of the white pulp in the spleen and HO-1-positive cells accumulated near the amyloid deposition area. CSPG was detected within the cells and also localized in the amyloid deposition area. CSPG was still not localized in the HO-1-positive cells. Double positive cells of HO-1 and CSPG were localized in the red pulp and in the amyloid deposition area on day 14. X-ray microanalysis indicated the existence of iron in the electron-dense bodies of fibroblasts in the amyloid deposition areas. The fibroblasts extended amyloid fibrils into the extracellular spaces of the marginal zone. These results suggest that HO-1-positive fibroblasts, but not HO-1-positive macrophages, are associated with the late stage of amyloid fibril formation.
...
PMID:Immunohistochemical detection of haem oxygenase in AA amyloidogenesis. 1558 41
Summary An adult female wild boar (Sus scrofa) was found moribund in Cabaneros National Park (central Spain). The animal had a markedly emaciated carcass, with body weight of 25.9 kg. At necropsy, most of the parenchymatous organs had widespread variably sized granulomas. Generalized tuberculosis was confirmed by PCR detection of
Mycobacterium
bovis in the mandibular lymph node. Large amounts of a hyaline, pale eosinophilic material were observed in liver, kidney and intestine. Congo red staining and green birefringence identified amyloid, which was further classified as AA type based on immunohistochemical results. It is speculated that the abundant
serum amyloid A
derivatives deposited in the tissues as AA-amyloid may be associated with the generalized tuberculosis. This is the first report of amyloidosis in the European wild boar.
...
PMID:Systemic AA-amyloidosis in a European wild boar (Sus scrofa) suffering from generalized tuberculosis. 1583 45
Differential stress/inflammatory responses were characterized at the mRNA and protein levels in mandibular lymph nodes (MLN) and oropharyngeal tonsils of European wild boars (Sus scrofa), naturally infected with
Mycobacterium
bovis. Suppression-subtractive hybridization combined with immunohistochemistry and/or quantitative real-time RT-PCR were used to identify and characterize abundant stress/inflammatory gene sequences differentially expressed in tuberculous (TB+) wild boars. Genes identified in MLN and tonsils corresponded to
serum amyloid A
, arginase I, osteopontin, lysozyme, annexin I, and heat shock proteins, respectively. Global protein patterns in MLN and tonsils were compared between TB+ and nontuberculous (TB-) boars by 2-DE and MALDI-TOF MS. Five proteins, including stress/inflammatory proteins annexin V, serum albumin, and apolipoprotein A1 were found at lower levels in MLN of TB+ boars. Manganese superoxide dismutase was found up-regulated in MLN of TB+ boars. Five proteins, including creatine kinase and MHC class II antigens were found up-regulated in tonsils of TB+ boars. These results demonstrated differential stress/inflammatory responses in wild boars naturally infected with M. bovis and suggest possible markers of tuberculosis in this species that may prove useful for future studies of host-pathogen interactions and for diagnostics and vaccine development.
...
PMID:Proteomic and transcriptomic analyses of differential stress/inflammatory responses in mandibular lymph nodes and oropharyngeal tonsils of European wild boars naturally infected with Mycobacterium bovis. 1716 76
Five acute-phase reactants-
serum amyloid A
(
SAA
), C-reactive protein (CRP), haptoglobin, albumin, and iron-were measured using commercially available assays in 110 healthy rhesus macaques (Macaca mulatta), and reference intervals were established for future use in health monitoring of this species. Reference intervals established were as follows:
SAA
, 29.5-87.7 mg/L; CRP, 0-17.5 mg/L; haptoglobin, 354.3-2,414.7 mg/ L; albumin, 36.1-53.0 g/L; and iron, 13.3-40.2 micromol/L. Furthermore, changes in the acute-phase reactants were studied in two additional groups of animals: eight rhesus macaques suffering from acute traumatic injuries and nine rhesus macaques experimentally infected with
Mycobacterium
tuberculosis reflecting a chronic active inflammation. In animals with inflammation,
SAA
and haptoglobin concentrations were moderately increased, while CRP increased more than 200-fold. In addition, marked decreases in albumin and iron concentrations were observed. These results show that
SAA
, CRP, and haptoglobin are positive acute-phase proteins, whereas albumin and iron are negative acute-phase reactants in rhesus macaques.
...
PMID:Acute-phase responses in healthy and diseased rhesus macaques (Macaca mulatta). 2500 Jun 91
Boreal woodland caribou (
Rangifer tarandus caribou
) are listed as threatened across Canada, and a basic understanding of their health status is lacking. From December 2012 to April 2013, we investigated multiple health indices for adult female boreal caribou (
n
=163) captured from seven herds in NE British Columbia, Canada. Health indices included physical characteristics, physiologic and trace mineral status, exposure to or infection with selected pathogens, and measures of chronic stress and inflammation, including
serum amyloid A
, haptoglobin, and hair cortisol concentration. Key findings were exposure to the bacterium
Erysipelothrix rhusiopathiae
in 14% of individuals, mild to severe hair loss associated with winter tick (
Dermacentor albipictus
) infestations in 76% of caribou from December to early February and 81% from late February to early April, and evidence of trace mineral deficiencies with 99% and 34% of individuals deficient in copper and selenium, respectively. Seroprevalence for exposure to selected pathogens was: alphaherpesvirus (63%), pestivirus (1%),
Besnoitia
spp. (60%), and
Neospora caninum
(2%). All animals were seronegative to
Brucella
spp. and
Toxoplasma gondii
.
Mycobacterium
avium
ssp.
paratuberculosis
was not detected in any fecal samples. Parasite eggs or larvae, including
Parelaphostrongylus andersoni
(36%),
Skrjabinema
spp. (1%)
,
Strongyle-type eggs (11%),
Moniezia-
type eggs (8%), and nematodirines (3%), were detected on fecal examination, but at low intensity. Blood biochemistry values and hair cortisol concentrations were within ranges previously reported in
Rangifer tarandus
sspp. Some significant differences among herds were noted, including antler morphology, exposure to
Besnoitia
spp., and concentrations of
serum amyloid A
, copper, cobalt, manganese, and iron.
...
PMID:HEALTH SURVEY OF BOREAL CARIBOU (
RANGIFER TARANDUS CARIBOU
) IN NORTHEASTERN BRITISH COLUMBIA, CANADA. 3060 90