SwePub - search: L773:1071 412X

Enumeration	Reference	Cover	Find
1.	Ahlin, A, et al. (author) Gamma interferon treatment of patients with chronic granulomatous disease is associated with augmented production of nitric oxide by polymorphonuclear neutrophils 1999 In: Clinical and diagnostic laboratory immunology. - 1071-412X. ; 6:3, s. 420-424 Journal article (peer-reviewed)
2.	Albert, MJ, et al. (author) Phagocytosis of Vibrio cholerae O139 Bengal by human polymorphonuclear leukocytes 1999 In: Clinical and diagnostic laboratory immunology. - 1071-412X. ; 6:2, s. 276-278 Journal article (peer-reviewed)
3.	Alexeyev, O A, et al. (author) Elevated levels of total and Puumala virus-specific immunoglobulin E in the Scandinavian type of hemorrhagic fever with renal syndrome. 1994 In: Clinical and diagnostic laboratory immunology. - 1071-412X. ; 1:3, s. 269-72 Journal article (peer-reviewed)abstract In a previous study, it was reported that the total immunoglobulin E (IgE) level was increased in patients with hemorrhagic fever with renal syndrome (HFRS). The aim of the present study was to investigate whether specific IgE is synthesized during the course of the disease. For this purpose, an epsilon-capture enzyme-linked immunosorbent assay was developed. A total of 72 patients with HFRS caused by Puumala virus were studied. Three different control groups were included: 20 blood donors, 20 patients with other viral diseases (influenza A and B virus, acute Epstein-Barr virus, and acute cytomegalovirus infections), and 5 subjects with high levels of total IgE (median, 1,070 kU/liter; range, 773 to 5,740 kU/liter). The levels of total IgE were significantly higher during the acute phase of HFRS than those of blood donors (P < 0.01) and of patients with other viral diseases (P < 0.001). All patients developed a specific IgE response (median, 55 arbitrary units; range 24 to 123 arbitrary units) in the acute phase of the disease, whereas in the different control groups no specific IgE was detectable. Both total and specific IgE levels decreased during convalescence compared with those during the acute phase of HFRS (P < 0.001 and P < 0.001, respectively). In conclusion, we have shown that both total and specific IgE levels are increased in patients with HFRS compared with levels in patients with other viral diseases. The possible pathogenetic role of the specific IgE response in HFRS is discussed.
4.	Ananieva, Olga, et al. (author) Immune responses to bile-tolerant Helicobacter species in patients with chronic liver diseases, a randomized population group, and healthy blood donors 2002 In: Clinical and Diagnostic Laboratory Immunology. - 1071-412X. ; 9:6, s. 1160-1164 Journal article (peer-reviewed)abstract Bile-tolerant Helicobacter species such as Helicobacter pullorum, Helicobacter bilis, and Helicobacter hepaticus are associated with hepatic disorders in animals and may be involved in the pathogenesis of chronic liver diseases (CLD) in humans. Antibody responses to cell surface proteins of H. pullorum, H. bilis, and H. hepaticus in serum samples from patients with CLD, a randomized population group, and healthy blood donors were evaluated by using enzyme linked immunosorbent assay (ELISA). The results were compared with the antibody responses to Helicobacter pylori. For analysis of a possible cross-reactivity between bile-tolerant Helicobacter species and H. pylori, sera from a subpopulation of each group were absorbed with a whole-cell extract of H. pylori and retested by ELISA. Results before absorption showed that the mean value of the ELISA units for H. pullorum was significantly higher in patients with CLD than in healthy blood donors (P = 0.01). Antibody reactivity to cell surface protein of H. hepaticus was also significantly higher in the CLD patients than in the healthy blood donors and the population group (P = 0.005 and P = 0.002, respectively). Following the absorption, antibody responses to H. pullorum decreased significantly in all three groups (P = 0.0001 for CLD patients, P = 0.0005 for the population group, and P < 0.0001 for the blood donors), indicating that cross-reactivity between H. pylori and other Helicobacter spp. occurs. The antibody responses to H. hepaticus and H. bilis in CLD patients remained high following absorption experiments compared to ELISA results before absorption. The significance of this finding requires further investigations.
5.	Ando, Y, et al. (author) Antibody production against hepatitis C virus core and nonstructural 3 proteins is highly sensitive to deficits in T-cell function 1997 In: Clinical and diagnostic laboratory immunology. - : American Society for Microbiology. - 1071-412X .- 1098-6588. ; 4:1, s. 104-106 Journal article (peer-reviewed)abstract The influence of suppression of CD4+ and CD8+ T cells on the humoral responses to hepatitis C virus (HCV) core and nonstructural 3 proteins was studied. An increasing viral burden cannot substitute for the lack of functional T cells in maintaining humoral HCV-specific responses.
6.	Bakhiet, M, et al. (author) A new cell enzyme-linked immunosorbent assay demonstrates gamma interferon suppression by beta interferon in multiple sclerosis 1999 In: Clinical and diagnostic laboratory immunology. - 1071-412X. ; 6:3, s. 415-419 Journal article (peer-reviewed)
7.	Bjöersdorff, Anneli, et al. (author) Isolation and characterization of two European strains of Ehrlichia phagocytophila of equine origin 2002 In: Clinical and Diagnostic Laboratory Immunology. - 1071-412X. ; 9:2, s. 341-343 Journal article (peer-reviewed)abstract We report the isolation and partial genetic characterization of two equine strains of granulocytic Ehrlichia of the genogroup Ehrlichia phagocytophila. Frozen whole-blood samples from two Swedish horses with laboratory-verified granulocytic ehrlichiosis were inoculated into HL-60 cell cultures. Granulocytic Ehrlichia was isolated and propagated from both horses. DNA extracts from the respective strains were amplified by PCR using primers directed towards the 16S rRNA gene, the groESL heat shock operon gene, and the ank gene. The amplified gene fragments were sequenced and compared to known sequences in the GenBank database. With respect to the 16S rRNA gene, the groESL gene, and the ank gene, the DNA sequences of the two equine Ehrlichia isolates were identical to sequences found in isolates from clinical cases of granulocytic ehrlichiosis in humans and domestic animals in Sweden. However, compared to amplified DNA from an American Ehrlichia strain of the E. phagocytophila genogroup, differences were found in the groESL gene and ank gene sequences.
8.	Brostrom, C, et al. (author) Low relative frequencies of CD26(+) CD4(+) cells in long-term nonprogressing human immunodeficiency virus type 1-infected subjects 1998 In: Clinical and diagnostic laboratory immunology. - 1071-412X. ; 5:5, s. 662-666 Journal article (peer-reviewed)
9.	Colque-Navarro, P, et al. (author) Antibody responses in patients with staphylococcal septicemia against two Staphylococcus aureus fibrinogen binding proteins: clumping factor and an extracellular fibrinogen binding protein 2000 In: Clinical and diagnostic laboratory immunology. - 1071-412X. ; 7:1, s. 14-20 Journal article (peer-reviewed)
10.	Cosma, A, et al. (author) Neutralization assay using a modified vaccinia virus Ankara vector expressing the green fluorescent protein is a high-throughput method to monitor the humoral immune response against vaccinia virus 2004 In: Clinical and diagnostic laboratory immunology. - 1071-412X. ; 11:2, s. 406-410 Journal article (peer-reviewed)
11.	Dahlbom, I, et al. (author) Immunoglobulin g (IgG) anti-tissue transglutaminase antibodies used as markers for IgA-deficient celiac disease patients 2005 In: Clinical and Diagnostic Laboratory Immunology. - 1071-412X. ; 12:2, s. 254-258 Journal article (peer-reviewed)abstract The role of immunoglobulin A (IgA) anti-tissue transglutaminase antibodies (IgA-tTG) as predictors of untreated celiac disease (CoD) is well documented, and the presence and levels of these antibodies are most accurately monitored with native or recombinant human antigens. However, IgA-deficient CoD patients are not identified by IgA serology, and conflicting results concerning the diagnostic validity of IgG antibodies against gliadin (IgG-AGA), endomysium (IgG-EmA), and tTG (IgG-tTG) have been reported. The aim of the present study was to evaluate the utility of IgG-tTG for the detection of CoD in IgA-deficient patients. Samples from 115 IgA-deficient and 200 IgA-sufficient subjects were collected and tested for the presence of IgA and IgG antibodies against tTG, EmA, and AGA. Antibodies against tTG were measured by an enzyme-linked immunosorbent assay based on recombinant human tTG, and antibodies against EmA were determined by immunofluorescence. The values for IgG-tTG showed a higher correlation (correlation coefficient [r] = 0.91) with those for IgG-EmA for the IgA-deficient subjects than for the IgA-sufficient subjects (r = 0.88). The overall concordance of the positive and negative results between IgG-tTG and IgG-EmA was 97%, and the IgG-tTG assay discriminated between IgG-EmA-positive and -negative subjects with IgA deficiency at a rate of 100%. Elevated levels of IgG-tTG and IgG-EmA were measured in 70% of the IgA-sufficient subjects. IgG-tTG detection with recombinant human tTG is a good alternative to IgG-EmA detection, and the addition of IgG-tTG assessment to present screening methods may improve the ability to identify IgA-deficient subjects with CoD.
12.	Du, Liping, et al. (author) Exposure of HEp-2 Cells to Stress Conditions Influences Antinuclear Antibody Reactivity. 2002 In: Clinical and Diagnostic Laboratory Immunology. - 1071-412X. ; 9:2, s. 287-294 Journal article (peer-reviewed)abstract This study of stress-related antinuclear antibody (ANA) reactivity was undertaken with the objective of improving clinical ANA testing. ANA was determined by parallel enzyme-linked immunosorbent assays of crude nuclear protein antigen extracted from HEp-2 cells either grown under optimal conditions (providing nonstress ANA antigen) or exposed to stress (providing stress ANA antigen). The stress stimuli used were gamma radiation (causing DNA damage) and a hypertonic environment (causing apoptosis). Signs of stress-related ANA reactivity were seen among connective tissue disease (CTD) patients (including patients with systemic lupus erythematosus; mixed CTD; calcinosis, Reynaud's phenomenon, esophageal motility disorders, sclerodactyly, and telangiectasia; scleroderma; and Sjögren's syndrome): 11% showed stress-positive ANA (i.e., a significantly stronger ANA reactivity with the extract from stressed cells), whereas 21% showed a markedly weaker reaction with the stress antigen. In contrast, among ANA screening patient sera, with no diagnosis of CTD, the fraction showing stress-positive ANA was higher (7 to 8%, depending on the type of stress) than among those showing a lower reactivity with stress antigen (1.5 to 2.5%). Only one serum among 89 (1%) tested sera from healthy individuals showed a stress-related ANA reaction. This demonstration of stress-related ANA suggests a means to improve the performance of clinical ANA testing.
13.	Elfaitouri, Amal, et al. (author) Quantitative PCR-Enhanced Immunoassay for Measurement of Enteroviral Immunoglobulin M Antibody and Diagnosis of Aseptic Meningitis. 2005 In: Clin Diagn Lab Immunol. - 1071-412X. ; 12:2, s. 235-41 Journal article (peer-reviewed)
14.	Enbom, M, et al. (author) Similar humoral and cellular immunological reactivities to human herpesvirus 6 in patients with multiple sclerosis and controls 1999 In: Clinical and diagnostic laboratory immunology. - 1071-412X. ; 6:4, s. 545-549 Journal article (peer-reviewed)
15.	Enroth, H, et al. (author) Clustering of clinical strains of Helicobacter pylori analyzed by two-dimensional gel electrophoresis 2000 In: Clinical and diagnostic laboratory immunology. - 1071-412X. ; 7:2, s. 301- Journal article (peer-reviewed)
16.	Eriksson, A, et al. (author) Streptococcal DNase B is immunologically identical to superantigen SpeF but involves separate domains 1999 In: Clinical and diagnostic laboratory immunology. - 1071-412X. ; 6:1, s. 133-136 Journal article (peer-reviewed)
17.	Ernerudh, Jan, 1952-, et al. (author) Effect of photopheresis on lymphocyte population in children with newly diagnosed type 1 diabetes 2004 In: Clinical and Diagnostic Laboratory Immunology. - 1071-412X. ; 11:5, s. 856-861 Journal article (peer-reviewed)abstract In recent years photopheresis has been claimed to be an effective form of immunomodulation. It has also been shown to have an effect on the disease process at the onset of type 1 diabetes. In a double-blind, placebo-controlled randomized study, we analyzed if the effect of photopheresis in children with newly diagnosed diabetes is related to changes in the balance of lymhocyte populations. We also analyzed if lymphocyte subsets were related to recent infection, mild or aggressive disease manifestations, heredity, or gender. Nineteen children received active treatment with photopheresis, while 21 children received sham pheresis (placebo group). No influence of a history of previous infection, heredity, or certain clinical parameters on lymphocyte subsets was found. At the onset of type 1 diabetes, girls showed a higher proportion and a larger number of T cells (CD3+) and T-helper cells (CD4+) and a higher proportion of naïve CD4 +CD45RA+ cells. In the placebo group, an increase in the number of subsets with the activated phenotype in both the CD4 (CD29 +) and the CD8 (CD11a+) compartments was noted during the course of the study. These changes did not occur in the photopheresis group. No relation between lymphocyte subsets and clinical outcome was found 1 year after the treatment with photopheresis. In conclusion, we found no major effect of photopheresis on lymphocyte populations in a group of children with newly diagnosed type 1 diabetes. However, in the placebo group the proportions of activated CD4 and CD8 cells increased over time. Since these changes did not occur in the actively treated group, our findings suggest that photopheresis may have some suppressive effects.
18.	Granert, C, et al. (author) The polysaccharide fucoidin inhibits the antibiotic-induced inflammatory cascade in experimental pneumococcal meningitis 1998 In: Clinical and diagnostic laboratory immunology. - 1071-412X. ; 5:3, s. 322-324 Journal article (peer-reviewed)
19.	Grodzinsky, Ewa, 1958-, et al. (author) New automated immunoassay measuring immunoglobulin A antigliadin antibodies for prediction of celiac disease in childhood. 2001 In: Clinical and diagnostic laboratory immunology. - 1071-412X. ; 8:3, s. 564-570 Journal article (peer-reviewed)
20.	Guzman, GE, et al. (author) Comparison between the skin snip test and simple dot blot assay as potential rapid assessment tools for Onchocerciasis in the postcontrol era in Ghana 2002 In: Clinical and diagnostic laboratory immunology. - 1071-412X. ; 9:5, s. 1014-1020 Journal article (peer-reviewed)
21.	Han, SR, et al. (author) vacA genotypes and genetic diversity in clinical isolates of Helicobacter pylori 1998 In: Clinical and diagnostic laboratory immunology. - 1071-412X. ; 5:2, s. 139-145 Journal article (peer-reviewed)
22.	Hoang, TTH, et al. (author) Seroprevalence of Helicobacter pylori infection in urban and rural Vietnam 2005 In: Clinical and diagnostic laboratory immunology. - 1071-412X. ; 12:1, s. 81-85 Journal article (peer-reviewed)
23.	Hultgren, C, et al. (author) Antibodies to the hepatitis B e antigen (HBeAg) can be induced in HBeAg-transgenic mice by adoptive transfer of a specific T-helper 2 cell clone 1997 In: Clinical and diagnostic laboratory immunology. - 1071-412X. ; 4:5, s. 630-632 Journal article (peer-reviewed)
24.	Iroegbu, J, et al. (author) Variability and immunogenicity of human immunodeficiency virus type 1 p24 gene quasispecies 2000 In: Clinical and diagnostic laboratory immunology. - 1071-412X. ; 7:3, s. 377-383 Journal article (peer-reviewed)
25.	Jaatinen, Taina, et al. (author) Total C4B deficiency due to gene deletion and gene conversion in a patient with severe infections 2003 In: Clinical and Diagnostic Laboratory Immunology. - 1071-412X. ; 10:2, s. 195-201 Journal article (peer-reviewed)abstract Deficiencies of the early components of the classical complement pathway impair the actions of innate and humoral immunity and may lead to increased susceptibility to infections. We have studied the genetic basis of total C4B deficiency in a Finnish patient with recurrent meningitis, chronic fistulas and abscesses. The maternal chromosome carried a four-gene deletion including the C4B gene, and a conversion from C4B to C4A gene was found on the paternal chromosome resulting in complete deficiency of C4B. In the converted C4A gene, mutation screening did not reveal any amino acid changes or prominent mutations, yet a large number of nucleotide variations were found. Further, the patient was heterozygous for structural deficiency of mannan binding lectin (MBL) associating with medium levels of serum MBL. Our data provides new information on the genetic instability of the C4 gene region, and on the association of homozygous C4B deficiency and variant MBL genotype with increased susceptibility to recurrent and chronic infections. Importantly, plasma therapy induced a prompt clinical cure with long-term effects.
26.	Jensenius, M, et al. (author) Comparison of immunofluorescence, Western blotting, and cross-adsorption assays for diagnosis of African tick bite fever 2004 In: Clinical and diagnostic laboratory immunology. - 1071-412X. ; 11:4, s. 786-788 Journal article (peer-reviewed)
27.	Kebede, T, et al. (author) Differences in humoral responses to the p24 antigen between Ethiopian and Swedish human immunodeficiency virus type 1-infected patients may suggest influences from a T-helper 2-like phenotype 1997 In: Clinical and diagnostic laboratory immunology. - 1071-412X. ; 4:5, s. 627-629 Journal article (peer-reviewed)
28.	Klintman, Daniel, et al. (author) Important role of p-selectin for leukocyte recruitment, hepatocellular injury, and apoptosis in endotoxemic mice. 2004 In: Clinical and Diagnostic Laboratory Immunology. - 1071-412X. ; 11:1, s. 56-62 Journal article (peer-reviewed)abstract Leukocyte recruitment in the liver includes a two-step procedure in which selectin-dependent leukocyte rolling is a prerequisite for subsequent CD18-dependent leukocyte firm adhesion in postsinusoidal venules. However, the roles of the individual selectins in leukocyte rolling and adhesion, hepatocellular injury, and apoptosis remain elusive. Therefore, we examined the pathophysiological role of P-, E-, and L-selectin in male C57BL/6 mice challenged with lipopolysaccharide (LPS) and D-galactosamine (Gal) by use of intravital microscopy of the liver microcirculation. In control animals, administration of LPS-Gal provoked reproducible hepatic damage, including marked increases of leukocyte recruitment, liver enzymes, and hepatocyte apoptosis and reduced sinusoidal perfusion. Interestingly, pretreatment with an anti-P-selectin antibody (RB40.34) markedly reduced leukocyte rolling and firm adhesion by 65 and 71%, respectively. Moreover, interference with P-selectin function significantly improved sinusoidal perfusion and reduced the increase in liver enzymes by 49 to 84% in endotoxemic mice. Moreover, the activity of caspase-3 and the number of apoptotic hepatocytes were significantly reduced by 55 and 54%, respectively, in RB40.34-treated animals. In contrast, administration of an anti-E-selectin antibody (10E9.6) and an anti-L-selectin antibody (Mel-14) did not protect against endotoxin-induced leukocyte responses or hepatic injury. In conclusion, our novel findings document a principal role of P-selectin in mediating leukocyte rolling, a precondition to the subsequent firm adhesion of leukocytes in liver injury. Furthermore, our novel data demonstrate that inhibition of P-selectin function reduces hepatocellular injury and apoptosis, suggesting a causal relationship between leukocyte recruitment on one hand and hepatocellular injury and apoptosis on the other hand. Based on these findings, it is suggested that P-selectin may be an important therapeutic target in endotoxin-induced liver injury.
29.	Kondori, Nahid, 1967, et al. (author) Circulating beta (1-3) glucan and immunoglobulin G subclass antibodies to Candida albicans cell wall antigens in patients with systemic candidiasis. 2004 In: Clinical and diagnostic laboratory immunology. - 1071-412X. ; 11:2, s. 344-50 Journal article (peer-reviewed)abstract Invasive candidiasis in patients who are immunocompromised or in intensive care units (ICUs) presents both diagnostic and therapeutic problems. We previously described antibodies that were directed against Candida albicans cell wall fragments (CW), periodate-treated CW (CW(IO4)), phosphopeptidomannan (PPM), and beta(1-3) glucan. In this study, circulating fungal antigens [mannan and beta(1-3) glucan] and immunoglobulin G (IgG) subclass antibodies to these cell wall antigens (anti-CW) were analyzed in patients with systemic candidiasis. Sera were collected from 14 patients on two or three consecutive occasions, starting on the day when candidiasis was culture proven. The sera were analyzed by enzyme-linked immunosorbent assay. The control groups consisted of lactating mothers (n = 9) (group I) who had breast milk that was positive for C. albicans and also had acute inflammation of the nipples, and age-matched blood donors (n = 10) (group II). Within the first 3 weeks of Candida infection all of the patients were positive for beta(1-3) glucan by the Gluspecy test, but no patients were positive for mannan in the less-sensitive Pastorex Candida test. The controls were negative for both beta(1-3) glucan (<20 pg/ml) and mannan (<2.5 ng/ml). IgG1 anti-CW and IgG2 anti-PPM antibodies were the most discriminatory antibodies. The ratio of IgG1 anti-CW to IgG2 anti-PPM was significantly lower in nonsurviving patients than in the other patients within the first week of candidiasis (P = 0.019). The IgG2 levels of anti-CW(IO4) and antiglucan antibodies correlated strongly (r = 0.681; P < 0.0001), and the absence of these antibodies was associated with increased levels of beta(1-3) glucan. Increased levels of IgG1 anti-CW or IgG2 anti-PPM antibodies (titer of > or = 3 logs) or of a combination of the two antibodies (log sum, > or = 5) showed 92% sensitivity, 100% specificity, and positive predictive values. In conclusion, beta(1-3) glucan and the two subclass antibodies appear to be early specific markers for the laboratory diagnosis of candidiasis. Furthermore, the kinetics of beta(1-3) glucan appearance in serum may assist in evaluating the therapeutic efficacy of antifungal treatments.
30.	Kouwenhoven, M, et al. (author) Enzyme-linked immunospot assays provide a sensitive tool for detection of cytokine secretion by monocytes 2001 In: Clinical and diagnostic laboratory immunology. - 1071-412X. ; 8:6, s. 1248-1257 Journal article (peer-reviewed)
31.	Kroca, Michal, et al. (author) Vγ9Vδ2 T cells in human legionellosis 2001 In: Clinical and diagnostic laboratory immunology. - 1071-412X. ; 8, s. 949-954 Journal article (peer-reviewed)
32.	La Scola, B, et al. (author) Serological differentiation of murine typhus and epidemic typhus using cross-adsorption and Western blotting 2000 In: Clinical and diagnostic laboratory immunology. - 1071-412X. ; 7:4, s. 612-616 Journal article (peer-reviewed)
33.	Lazzarotto, T, et al. (author) Evaluation of the Abbott AxSYM cytomegalovirus (CMV) immunoglobulin M (IgM) assay in conjunction with other CMV IgM tests and a CMV IgG avidity assay 2001 In: Clinical and diagnostic laboratory immunology. - 1071-412X. ; 8:1, s. 196-198 Journal article (peer-reviewed)
34.	Levi, M, et al. (author) Peptide sequences of glycoprotein G-2 discriminate between herpes simplex virus type 2 (HSV-2) and HSV-1 antibodies 1996 In: Clinical and diagnostic laboratory immunology. - 1071-412X. ; 3:3, s. 265-269 Journal article (peer-reviewed)
35.	Lopes, Ana I, et al. (author) Cytokine expression in pediatric Helicobacter pylori infection. 2005 In: Clinical and diagnostic laboratory immunology. - 1071-412X. ; 12:8, s. 994-1002 Journal article (peer-reviewed)abstract Helicobacter pylori infection is one of the most common gastrointestinal infections worldwide and almost invariably causes chronic gastritis in the infected host. A predominant Th1 profile has been demonstrated in H. pylori-infected mucosa from adults, but no previous study has evaluated in situ cytokine expression in children. We therefore examined expression of proinflammatory, anti-inflammatory, and regulatory cytokines by immunohistochemistry in cryopreserved antral biopsy specimens from 10 H. pylori-infected and 10 uninfected children and correlated expression of cytokines with histology scores. Concomitant expression of interleukin-8 (IL-8), gamma interferon (IFN-gamma), IL-4, transforming growth factor beta, and tumor necrosis factor alpha was seen in 8/10 H. pylori-infected cases and in 5/10 noninfected cases; all H. pylori-infected subjects showed staining for at least two of the cytokines. The proportion of epithelial cytokine-specific staining did not differ significantly between the groups, either in surface or glandular epithelium. Furthermore, no significant differences were noticed between intraepithelial or lamina propria lymphocyte staining in the groups. There was, however, a tendency of higher numbers of IFN-gamma- and IL-8-positive cells in the H. pylori-infected group. IFN-gamma and IL-8 lamina propria lymphocyte expression correlated significantly with antrum chronic inflammation, but there was no correlation between histology scores and epithelial cytokine expression. When the same techniques were used, the cytokine response appeared to be smaller in H. pylori-infected children than in adults, and there was no clear Th1 dominance. These results therefore suggest a different mucosal immunopathology in children. It remains to be determined whether the gastric immune response is downregulated in children with H. pylori infection and whether this is relevant to the outcome of infection.
36.	LUNDKVIST, A, et al. (author) Mapping of B-cell determinants in the nucleocapsid protein of Puumala virus: definition of epitopes specific for acute immunoglobulin G recognition in humans 1995 In: Clinical and diagnostic laboratory immunology. - 1071-412X. ; 2:1, s. 82-86 Journal article (peer-reviewed)
37.	Mattsson, Eva, et al. (author) Peptidoglycan Induces Mobilization of the Surface Marker for Activation Marker CD66b in Human Neutrophils but Not in Eosinophils. 2003 In: Clinical and Diagnostic Laboratory Immunology. - 1071-412X. ; 10:3, s. 485-488 Journal article (peer-reviewed)abstract Peptidoglycan from Staphylococcus aureus mobilized CD66b in human neutrophils but did not upregulate surface activation markers in eosinophils. In addition, Toll-like receptor 2, implicated in the recognition of peptidoglycan, was detected on the surface of resting neutrophils but not on eosinophils. These findings suggest roles for neutrophils but not eosinophils in innate recognition of peptidoglycan.
38.	Ohlin, Mats, et al. (author) Cytomegalovirus glycoprotein B-specific antibody analysis using electrochemiluminescence detection-based techniques 1997 In: Clinical and Diagnostic Laboratory Immunology. - 1071-412X. ; 4:1, s. 107-111 Journal article (peer-reviewed)abstract An electrochemiluminescence technique was used to develop versatile and sensitive assay strategies for determination of seroreactivities against biologically important cytomegalovirus neutralization epitopes expressed on glycoprotein B. Indirect binding assays showed wide linear assay ranges and revealed that serum samples diluted in parallel with a monoclonal antibody-based standard, simplifying quantitative analytical assessments.
39.	Ohlin, M., et al. (author) Human antibody reactivity against the lower matrix protein (pp65) produced by cytomegalovirus 1995 In: Clinical and Diagnostic Laboratory Immunology. - 1071-412X. ; 2:3, s. 325-329 Journal article (peer-reviewed)abstract The lower matrix protein (pp65) is a major product of many laboratory strains of cytomegalovirus (CMV). It is thus an integral part of many CMV serological assays based on native antigen. Recombinant fragments of pp65 have previously been investigated for their usefulness in more-defined assays. The latter antigens have, however, failed to develop a positive response with serum samples derived from a substantial number of infected individuals. Here we show that the human humoral immune response to CMV pp65 is highly diverse and recognizes at least seven distinct but in some cases partly overlapping epitopes. Most of these epitopes could not be mimicked by any of the investigated recombinant or synthetic antigens. Furthermore, when we investigated the ability of human CMV-seropositive serum samples to block the reactivity of pp65 specific antibodies recognizing five different epitopes within pp65, it was evident that several sera did not contain significant levels of antibodies against any of these or overlapping structures. It was thus concluded that the antibody response against CMV pp65 is weak in some CMV-infected individuals, making this antigen unsuitable for use alone in serological screening systems for CMV infection.
40.	Ornstein, Katharina, et al. (author) Differential immune response to the variable surface loop antigen of P66 of Borrelia burgdorferi sensu lato species in geographically diverse populations of lyme borreliosis patients 2002 In: Clinical and diagnostic laboratory immunology. - 1071-412X. ; 9:6, s. 1382-1384 Journal article (peer-reviewed)abstract We have studied the immune response to a variable surface-exposed loop region of the P66 outer membrane protein from Borrelia burgdorferi sensu lato by using an enzyme immunoassay. Lyme borreliosis populations found in North America and Sweden were preferentially more seroreactive to P66 from their respective regional species, namely, B. burgdorferi sensu stricto and B. garinii and B. afzelii, respectively.
41.	Pilch, H, et al. (author) Antigen-driven T-cell selection in patients with cervical cancer as evidenced by T-cell receptor analysis and recognition of autologous tumor 2002 In: Clinical and diagnostic laboratory immunology. - 1071-412X. ; 9:2, s. 267-278 Journal article (peer-reviewed)
42.	Pussinen, PJ, et al. (author) Periodontitis is associated with a low concentration of vitamin C in plasma. 2003 In: Clinical and Diagnostic Laboratory Immunology. - 1071-412X. ; 10:5, s. 897-902 Journal article (peer-reviewed)abstract This study aimed to clarify how concentrations of vitamin C in plasma relate to the serology of periodontitis. The random sample used comprised 431 men, 194 from Finland and 237 from Russia. The plasma vitamin C concentration was determined by o-phtaldialdehyde-fluorometry, and serum immunoglobulin G antibodies to Actinobacillus actinomycetemcomitans and Porphyromonas gingivalis were determined by a multiserotype enzyme-linked immunosorbent assay (ELISA). The mean plasma vitamin C concentration was higher (P < 0.001) in Finnish subjects (mean +/- standard deviation, 4.5 +/- 2.8 mg/liter) than in Russian subjects (1.4 +/- 1.8 mg/liter). Mean antibody levels to both A. actinomycetemcomitans (4.7 +/- 3.6 versus 5.2 +/- 3.1 ELISA units [P = 0.05]) and P. gingivalis (5.7 +/- 2.5 versus 7.6 +/- 2.9 ELISA units [P < 0.001]) were lower in Finnish men than in Russian men. In the combined Finnish and Russian population, the antibody levels to P. gingivalis were negatively correlated with vitamin C concentrations (r = -0.22; P < 0.001); this association remained statistically significant (P = 0.010) in a linear regression model after adjustment for confounding factors. The proportion of P. gingivalis-seropositive subjects decreased with increasing vitamin C concentrations (P for trend, <0.01), but no trend was seen among A. actinomycetemcomitans-seropositive subjects. In conclusion, P. gingivalis infection is associated with low concentrations of vitamin C in plasma, which may increase colonization of P. gingivalis or disturb the healing of the infected periodontium.
43.	Rang, CU, et al. (author) Estimation of growth rates of Escherichia coli BJ4 in streptomycin-treated and previously germfree mice by in situ rRNA hybridization 1999 In: Clinical and diagnostic laboratory immunology. - 1071-412X. ; 6:3, s. 434-436 Journal article (peer-reviewed)
44.	Raqib, R, et al. (author) Use of antibodies in lymphocyte secretions for detection of subclinical tuberculosis infection in asymptomatic contacts 2004 In: Clinical and diagnostic laboratory immunology. - 1071-412X. ; 11:6, s. 1022-1027 Journal article (peer-reviewed)
45.	Rauprich, P, et al. (author) Influence of modified natural or synthetic surfactant preparations on growth of bacteria causing infections in the neonatal period 2000 In: Clinical and diagnostic laboratory immunology. - 1071-412X. ; 7:5, s. 817-822 Journal article (peer-reviewed)
46.	Rekabdar, Elham, 1971, et al. (author) Variability of the glycoprotein G gene in clinical isolates of herpes simplex virus type 1. 1999 In: Clinical and diagnostic laboratory immunology. - 1071-412X. ; 6:6, s. 826-31 Journal article (peer-reviewed)abstract Glycoprotein G (gG) of herpes simplex virus type 1 (HSV-1) has been used as a prototype antigen for HSV-1 type-specific serodiagnosis, but data on the sequence variability of the gene coding for this protein in wild-type strains are lacking. In this study, direct DNA sequencing of the gG-1 genes from PCR products was performed with clinical HSV-1 isolates from 11 subjects as well as with strains Syn 17(+), F, and KOS 321. The reference strains Syn 17(+) and F showed a high degree of conservation, while KOS 321 carried 13 missense mutations and, in addition, 12 silent mutations. Three clinical isolates showed mutations leading to amino acid alterations: one had a mutation of K(122) to N, which is a gG-1-to-gG-2 alteration; another contained all mutations which were observed in KOS 321 except two silent mutations; and the third isolate carried five missense mutations. Two clinical isolates as well as strain KOS 321 showed a mutation (F(111)-->V) within the epitope of a gG-1-reactive monoclonal antibody (MAb). When all viruses were tested for reactivity with the anti-gG-1 MAb, the three strains with the F(111)-->V mutation were found to be unreactive. Furthermore, gG-1 antibodies purified from sera from the two patients carrying strains mutated in this epitope were less reactive when they were tested by an HSV-1-infected-cell assay. Therefore, our finding that the sequence variability of the gG-1 gene also affects B-cell epitope regions of this protein in clinical isolates may have consequences for the use of this protein as a type-specific antigen for serodiagnosis.
47.	Riesbeck, Kristian, et al. (author) Endothelial cells expressing an inflammatory phenotype are lysed by superantigen-targeted cytotoxic T cells 1998 In: Clinical and Diagnostic Laboratory Immunology. - 1071-412X. ; 5:5, s. 675-682 Journal article (peer-reviewed)abstract The objective of this study was to investigate whether the superantigen staphylococcal enterotoxin A (SEA), which binds to HLA class II and T-cell receptor Vβ chains, can direct cytotoxic T cells to lyse cytokine-stimulated endothelial cells (EC). In addition, we wanted to determine whether SEA- primed cytotoxic T cells could be targeted to EC surface molecules as a means of a novel cancer immunotherapy. Human umbilical vein EC (HUVEC), dermal microvascular EC (HMVEC), or the EC line EA.hy926 stimulated with gamma interferon (IFN-γ) or tumor necrosis factor alpha (TNF-α) displayed upregulated HLA class II and adhesion molecule (CD54 and CD106) expression, respectively. SEA-primed T cells induced a strong cytotoxicity against IFN- γ,- and TNF-α-activated EA.hy926 which had been preincubated with SEA. Blocking of CD54 completely abrogated the T-cell attack. SEA-D227A, which has a mutated class II binding site, did not promote any cytotoxicity. A strong lysis was observed when a fusion protein consisting of protein A and SEA- D227A was added together with T cells to TNF-α-induced EA.hy926 and HUVEC precoated with monoclonal antibodies (MAb) directed against HLA class I, CD54, or CD106 molecules. Finally, an scFv antibody fragment reactive with an unknown EC antigen was fused with SEA-D227A. Both EA.hy926 and HMVEC were efficiently lysed by scFv-SEA-D227A-triggered cytotoxic T cells. Taken together, superantigen-activated T-cell-dependent EC killing was induced when EC expressed an inflammatory phenotype. Moreover, specific MAb targeting of the superantigen to surface antigens induced EC lysis. Our data suggest that directed T-cell-mediated lysis of unwanted proliferating EC, such as those in the tumor microvasculature, can be clinically useful.
48.	SAMUELSON, A, et al. (author) Characterization of the recognition site and diagnostic potential of an enterovirus group-reactive monoclonal antibody 1995 In: Clinical and diagnostic laboratory immunology. - 1071-412X. ; 2:3, s. 385-386 Journal article (peer-reviewed)
49.	Segelmark, Mårten, et al. (author) Monitoring proteinase 3 antineutrophil cytoplasmic antibodies for detection of relapses in small vessel vasculitis. 2003 In: Clinical and Diagnostic Laboratory Immunology. - 1071-412X. ; 10:5, s. 769-774 Journal article (peer-reviewed)
50.	Simán, Henrik, et al. (author) Evaluation of western blot CagA seropositivity in Helicobacter pylori-seropositive and -seronegative subjects. 2005 In: Clin Diagn Lab Immunol. - 1071-412X. ; 12:2, s. 304-309 Journal article (peer-reviewed)

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