Your search keyword '"Del Prete G"' showing total 14 results

1. In vitro production of IgE by human peripheral blood mononuclear cells II. CELLS INVOLVED IN THE SPONTANEOUS IgE PRODUCTION IN ATOPIC PATIENTS.

Author

Romagnani, S., Del Prete, G. F., Maggi, E., Troncone, R., Giudizi, Grazia M., Almerigogna, F., and Ricci, M.

Subjects

*MONONUCLEOSIS, *LYMPHOCYTES, *T cells, *LEUCOCYTES, *PLASMA cells, *LYMPHOID tissue

Abstract

Spontaneous IgE production in vitro was investigated in 7-day cultures of unfractionated mononuclear cells (MNC) and MNC subpopulations from atopic patients. Depletion of either phagoctytic or adherent cells decreased the amount of IgE detectable in 7-day culture supernatants, but this decrease was due, at least in part, to a loss of cytophilic IgE. Depletion of immunoglobulin-bearing cells (SIg+) reduced significantly but did not abolish the spontaneous IgE production in vitro. On the other hand, depletion of IgM- bearing lymphocytes (SIgM+) which virtually abolished the production of immunoglobulins of the IgM class, did not change significantly the spontaneous production of IgE. Similarly, no change in the spontaneous production of IgE was found when lymphocyte suspensions were depleted of complement receptor-bearing cells (CR+). In contrast. spontaneous IgE product ion was significantly increased by depict ion of T lymphocytes and this increase did not simply reflect the enrichment for IgE-producing cells caused by the fractionation procedure. No significant change in the spontaneous IgE production was found when small numbers of autologous T lymphocytes were added to B cell fractions, whereas the addition of higher concentrations of autologous T cells induced a marked inhibition of the spontaneous IgE production. On the other hand, the addition in culture of pokeweed mitogen (PWM) resulted in a marked reduction of the spontaneous IgE production by B cells, also in the presence of small concentrations autologous T lymphocytes. Normal T cells were consistently effective in inducing a partial inhibition of the spontaneous IgE production by B cells from atopic patients. whereas T cells from a noticeable proportion of atopic patients were not. These data suggest that MNC responsible for the spontaneous IgE production in atopic subjects arc SIgM- and CR-deficient well-differentiated lymphocytes which probably represent the result of an activation which has occurred in vivo. However, this spontaneous IgE production can still be influenced by in vitro manipulation. such as variations in T-B cell ratios or addition of PWM. The results here reported also indicate that normal T cells arc generally more effective than T cells from atopic patients in regulating the activity of spontaneous IgE-producing cells present in the blood of atopic subjects. [ABSTRACT FROM AUTHOR]

Published

1980

2. Direct induction of human B-cell differentiation by recombinant interleukin-2.

Author

Romagnani, S., Del Prete, G., Giudizi, Maria O., Biagiotti, Roberta, Almerigogna, F., Tiri, A., Alessi, Anna, Mazzetti, M., and Ricci, M.

Subjects

*INTERLEUKINS, *B cell differentiation, *INTERLEUKIN-2, *B cells, *CELL differentiation, *CELL culture

Abstract

Recombinant interleukin-2 (rIL-2) induced highly purified human tonsillar B cells to differentiate into immunoglobulin (Ig)-producing cells in vitro. The B-cell response was not due to rIL-2- contaminating substances, but reflected the activity of IL-2 itself, since it was inhibited by addition to the cultures of anti-TAC monoclonal antibody. The rIL-2-induced B-cell response was apparently not mediated by factors released by residual T cells present in B-cell suspensions at undetectable levels, since supernatants (SN) from unstimulated autologous T cells cultured at concentrations even much higher than those possibly contaminating B-cell suspensions did not induce any detectable Ig production. In addition, the Ig production by B cells cultured with SN prepared from high numbers of autologous T cells stimulated with rIL-2, as well as from allo-activated or mitogen-stimulated T cells, was of the same magnitude as the Ig production resulting from direct addition of rIL-2 concentrations comparable with those present in the supernatants. After centrifugation on Percoll density gradients, most of the tonsillar B cells responsive to rIL-2 were recovered in the lower density cell fraction containing a number of larger activated B cells. Moreover, B-cell enriched suspensions from peripheral blood (PB) (which usually contains a lower number of in vivo activated B cells than tonsil) showed poor or no response to rIL-2 alone, but displayed significant Ig production when rIL-2 was added to the cultures in the presence of Staphylococcus aureus Cowan I (SAC) bacteria. Taken together, these data indicate that IL-2 can directly induce differentiation into Ig-producing cells of in vivo or in vitro activated human B cells. [ABSTRACT FROM AUTHOR]

Published

1986

3. T cell clones providing helper function for IgE synthesis release soluble factor(s) that induce IgE production in human B cells: possible role for interleukin 4 (IL-4).

Author

Maggi, E., Del Prete, G. F., Tiri, A., Macchia, Donatella, Parronchi, Paola, Ricci, M., and Romagnani, S.

Subjects

*T cells, *CLONING, *TONSILS, *B cells, *INTERLEUKINS, *INTERLEUKIN-4

Abstract

We have previously demonstrated that a proportion of human T cell clones (TCC) derived from tonsil or peripheral blood (PB) of non-allergic donors, upon triggering with phytohaemagglutinin (PHA) or anti-CD3 monoclonal antibody (MoAb), were able to provide help for IgE synthesis in B cells from both allergic and non-allergic individuals. In this study we show that, upon PHA stimulation, culture supernatants from 10 selected TCC active on IgE synthesis also provided helper activity for IgE, whereas supernatants from unstimulated cultures of the same TCC were ineffective. In contrast, culture supernatants derived from five PHA-stimulated TCC, unable to provide helper function for IgE synthesis, consistently failed to elicit production of IgE. While the induction of IgE synthesis by TCC occurred in B cells from virtually all allergic and non-allergic donors, their soluble factor(s) were found to be able to provide substantial help for IgE production only in B cells from a proportion of donors tested. In addition B cells from non-atopic donors usually appeared to be less responsive than atopic B cells to the activity of such factor(s). In contrast, synthesis of both IgG and IgM was induced in every B cell donor by both TCC and their supernatants. Partial characterization of the factor(s) providing helper function for IgE synthesis in B cells showed that it apparently had a mol. wt between 10 and 50 kD and did not bind to immobilized IgE. Such an activity appeared to be associated with the presence of interleukin 4 (IL-4) in supernatants and it was inhibited by adding both gamma-interferon and anti-human IL-4 antibody in culture. [ABSTRACT FROM AUTHOR]

Published

1988

4. Enhanced production of γ-interferon by thyroid-derived T cell clones from patients with Hashimoto's thyroiditis.

Author

Del Prete, G. F., Itri, A., Mariotti, S., Pinchera, A., Ricci, M., and Romagnani, S.

Subjects

*T cells, *LYMPHOCYTES, *ANTIVIRAL agents, *LYMPHOID tissue, *IMMUNE response, *BIOLOGICAL transport

Abstract

T lymphocytes from thyroid infiltrate and peripheral blood (PB) of four patients with Hashimoto's thyroiditis (HT) were analysed at clonal level for their ability to secrete interleukin 2 (IL-2) and y-interferon (y-IFN), As controls, T cell clones from PB of four normal donors and from spleen of two trauma victims were used. While no abnormality was found in the capacity lo produce lL-2, the proportion of y-IFN-producing (IFN-P) T cell clones derived from HT infiltrates was significantly higher (p<0-0005) than that of IFN-P clones derived from normal or patient PB. Most of CD4 +and CD8 + IFN-P clones from thyroid infiltrates, as well as a proportion of CD4 + PB-derived clones of patients with HT, released higher amounts of v-IFN than control clones. A relationship could be demonstrated between high y-IFN production and natural killer (NK) activity in T cell clones from thyroid and PB of HT patients. In fact, the percentage of I FN-P clones with NK potential (NK + ) was remarkably higher (p<0.0005) in thyroid infiltrates than in normal spleen or PB. The proportion of IFN-P NK + clones from patient PB was also significantly increased (P<0.02) but, unlike thyroid-derived clones in which the majority of IFN-P NK + clones were CD8 +, most PB-derived IFN-P NK + clones from the same patients expressed the CD4 + phenolype. Almost all thyroid NK + clones could be triggered to produce more y-IFN, while y-IFN synthesis by NK-negative thyroid clones was comparable to that of control clones. In view of the multiple effects ascribed to y-IFN in the cascade of events leading to immune responses, the abnormal potential to y-lFN secretion shown by intrathyroidal T lymphocytes may be of importance in the pathogenesis of autoimmune throiditis. [ABSTRACT FROM AUTHOR]

Published

1987

5. In vivo activated cytotoxic T cells in the thyroid infiltrate of patients with Hashimoto's thyroiditis.

Author

Del Prete, G. F., Vercelli, Donata, Tiri, A., Maggi, E., Mariotti, S., Pinchera, A., Ricci, M., and Romagnani, S.

Subjects

*AUTOIMMUNE thyroiditis, *T cells, *LYMPHOCYTES, *ANTIGENS, *MOLECULAR cloning, *ENDOCRINE glands

Abstract

High proportions of T8+ cells with inverted T4/T8 ratio were found in freshly isolated thyroid lymphocytes from patients with Hashimoto's thyroiditis. In addition, about one third of thyroid infiltrating cells expressed the TAC antigen, whereas in patient peripheral blood (PB) or normal lymphocytes from PB or lymphoid organs the percentage of TAC-positive cells was consistently lower than 10%. Following negative selection with OKT4 or OKT8 monoclonal antibodies and complement, TAC+ T cells were enriched in the T8+ cell population. Thyroid infiltrating T cells from two patients underwent two different cloning procedures. In the first, single T cells were initially activated with phytohaemagglutinin (PHA) and interleukin 2 (IL-2), in the other with recombinant IL-2 (rIL-2) alone. The majority of T cell clones obtained by initial PHA-stimulation (55 - 65%) had the T8+ phenotype, but the frequency of T8+ clones obtained by stimulating T cells with rIL-2 alone was even higher (78 & 71%, respectively). The majority of T8+ clones elicited by PHA (35/37 & 36/38) and all the T8+ clones (36/ 36 & 22/22) obtained from thyroid infiltrates with initial stimulation by rIL-2 displayed cytolytic activity, Most of cytolytic T8+ clones obtained from thyroid infiltrates with both cloning procedures, displayed NK activity against human K562and MOLT-4 target cells, but not against a NK-resistant target, such as Raji cells. These data suggest that in Hashimoto's disease a considerable proportion of thyroid infiltrating T cells are in vivo activated T8+ cytolytic T cells with N K activity, which may be of importance in determining or maintaining the tissue damage of the target gland. [ABSTRACT FROM AUTHOR]

Published

1986

6. Role for T cells, IL-2 and IL-6 in the IL-4-dependent <em>in vitro</em> human IgE synthesis.

Author

Maggi, E., del Prete, G. F., Parrochi, P., Tiri, A., Macchia, D., Biswas, P., Simonelli, C., Ricci, M., and Romagnani, S.

Subjects

*T cells, *MONOCYTES, *CYTOKINES, *INTERLEUKINS, *B cells, *IMMUNOGLOBULIN E

Abstract

The role of T cells and monocytes, as well as that of cytokines, such as IL-I, IL-2 and IL-6, on the IL-4-dependent in vitro human IgE synthesis was investigated. Recombinant IL-4, IL-4-containing T-cell clone supernatants and different combinations of recombinant cytokines failed to induce highly purified B cells to synthesize IgE. IL-4-dependent IgE synthesis was restored by addition to purified B cells of either untreated or mitomycin C-treated autologous T lymphocytes. Addition to purified B cells of autologous monocytes did not restore the IgE response, but usually it exerted a potentiating effect on the synthesis of IgE induced by IL-4 in the presence of suboptimal concentrations of T cells. The activity of T cells apparently preceded that of IL-4 and required a physical contact with B cells. The presence in culture of IL-2 also appeared to be necessary for the T-cell and IL-4-depeodent IgE synthesis. Even though not essential, IL-6 was able to potentiate IgE synthesis in most experimentS, whereas IL-I did not display any modulatory effect. [ABSTRACT FROM AUTHOR]

Published

1989

7. IgE Synthesis in vitro induced by T cell factors from patients with elevated serum IgE levels.

Author

Romagnani, S., Maggi, E., del Prete, G. F., and Ricci, M.

Subjects

*IMMUNOGLOBULIN E, *ATOPIC dermatitis, *CELL culture, *T cells, *SKIN inflammation, *CULTURES (Biology)

Abstract

The effect of unstimulated T cell culture supernatants (TCS) from patients with atopic dermatitis and high serum IgE levels on the IgE production in vitro by B cell rich suspensions from normal individuals or grass pollen sensitive patients with mild atopy was evaluated. TCS from patients with raised IgE enabled B cell suspensions from normal individuals to produce detectable amounts of IgE and potentiated the spontaneous IgE synthesis in vitro by B cell suspensions from grass sensitive patients. In contrast, the addition of TCS from normal subjects with low serum IgE levels did not increase or even reduced IgE synthesis by B cell cultures. When the same B cell cultures were analysed for their ability to produce IgG or IgM protein, no significant differences were observed. These findings indicate that T lymphocytes from patients with high serum IgE levels can release soluble factor(s) possessing isotype (IgE) specific potentiating activity. [ABSTRACT FROM AUTHOR]

Published

1983

8. In vitro production of IgE by human peripheral blood mononuclear cells.

Author

Romagnani, S., Maggi, E., Del Prete, G. F., Troncone, R., and Ricci, M.

Subjects

*IMMUNOGLOBULIN E, *PROTEINS, *IMMUNOGLOBULINS, *POKEWEED mitogens, *PLANT lectins, *AMINOGLYCOSIDES

Abstract

IgE protein and grass-specific IgE antibodies were detected in the supernatants of 7-day cultures of unstimulated and pokeweed mitogen (PWM) stimulated human blood mononuclear cells from non-atopic and grass pollen-sensitive individuals. Significant amounts of IgE protein were detected in culture supernatants of grass-sensitive individuals and, even at lower levels, in those of non-atopic subjects In contrast, detectable amounts of grass-specific antibodies were found only in the culture supernatants of grass-sensitive subjects. The mean values of total and grass-specific IgE detected in the supernatants of unstimulated and PWM-stimulated cultures did not differ statistically. Time sequence studies showed that IgE concentrations, measured in the 7-day supernatants. were due to a continuous release from the cells of IgE quantities progressively decreasing up to days 7 or 8. Comparison of the IgE protein and IgE antibody found in the 7-dayculturesupernatants to those released from initial cell pellets by treatment with acid buffer or freezing and thawing, showed that the IgE detected in 7-day supernatants could result, in part, from the release of cytophilic IgE bound to basophil or other cell types and in part also from the release of preformed lymphocyte cytoplasmic IgE into the supernatant fluids during the course of culture. In most non-atopic subjects and in some grass-sensitive patients the preformed IgE accounted virtually for the total IgE detected in the 7-day culture supernatants. However, the increase of IgE above the levels measured in the initial cell pellets, which was found inmost grass-sensitive subjects, clearly reflected newly synthesized IgE. Both cycloheximide and puromycin were capable of reducing significantly the IgE concentration in culture supernatants when it was greater than the amount found in the initial cell pellets. The treatment of cells with mitomycin C was also able to decrease significantly the amount of IgE released in the supernatant after day 3 of culture. [ABSTRACT FROM AUTHOR]

Published

1980

9. Nucleic Acid, Antibody, and Virus Culture Methods to Detect Xenotropic MLV-Related Virus in Human Blood Samples.

Author

Kearney, M. F., Lee, K., Bagni, R. K., A. Wiegand,, A., Spindler, J., Maldarelli, F., Pinto, P. A., Linehan, W. M., Vocke, C. D., Delviks-Frankenberry, K. A., de VereWhite, R. W., Del Prete, G. Q., Mellors, J. W., Lifson, J. D., KewalRamani, V. N., Pathak, V. K., Coffin, J. M., and Le Grice, S. F. J.

Subjects

*MOUSE leukemia viruses, *NUCLEIC acids, *VIRAL antibodies, *BLOOD testing, *RETROVIRUS diseases, *DIAGNOSIS, *PROSTATE cancer, *CHRONIC fatigue syndrome

Abstract

The MLV-related retrovirus, XMRV, was recently identified and reported to be associated with both prostate cancer and chronic fatigue syndrome. At the National Cancer Institute-Frederick, MD (NCI-Frederick), we developed highly sensitive methods to detect XMRV nucleic acids, antibodies, and replication competent virus. Analysis of XMRV-spiked samples and/or specimens from two pigtail macaques experimentally inoculated with 22Rv1 cell-derived XMRV confirmed the ability of the assays used to detect XMRV RNA and DNA, and culture isolatable virus when present, along with XMRV reactive antibody responses. Using these assays, we did not detect evidence of XMRV in blood samples (N = 134) or prostate specimens (N = 19) from two independent cohorts of patients with prostate cancer. Previous studies detected XMRV in prostate tissues. In the present study, we primarily investigated the levels of XMRV in blood plasma samples collected from patients with prostate cancer. These results demonstrate that while XMRV-related assays developed at the NCI-Frederick can readilymeasure XMRV nucleic acids, antibodies, and replication competent virus, no evidence of XMRV was found in the blood of patients with prostate cancer. [ABSTRACT FROM AUTHOR]

Published

2011

10. Borrelia burgdorferi NapA-driven Th17 cell inflammation in lyme arthritis.

Author

Codolo G, Amedei A, Steere AC, Cappon A, Papinutto E, Polenghi A, Benagiano M, Paccani SR, Sambri V, Del Prete G, Baldari CT, Zanotti G, Montecucco C, D'Elios MM, and de Bernard M

Abstract

OBJECTIVE: Human Lyme arthritis caused by Borrelia burgdorferi is characterized by an inflammatory infiltrate that consists mainly of neutrophils and T cells. This study was undertaken to evaluate the role of the innate and acquired immune responses elicited by the neutrophil-activating protein A (NapA) of B burgdorferi in patients with Lyme arthritis. METHODS: Serum anti-NapA antibodies were measured in 27 patients with Lyme arthritis and 30 healthy control subjects. The cytokine profile of synovial fluid T cells specific for NapA was investigated in 5 patients with Lyme arthritis. The cytokine profile induced by NapA in neutrophils and monocytes was also investigated. RESULTS: Serum anti-NapA antibodies were found in 48% of the patients with Lyme arthritis but were undetectable in the healthy controls. T cells from the synovial fluid of patients with Lyme arthritis produced interleukin-17 (IL-17) in response to NapA. Moreover, NapA was able to induce the expression of IL-23 in neutrophils and monocytes, as well as the expression of IL-6, IL-1beta, and transforming growth factor beta (TGFbeta) in monocytes, via Toll-like receptor 2. CONCLUSION: These findings indicate that NapA of B burgdorferi is able to drive the expression of IL-6, IL-1beta, IL-23, and TGFbeta by cells of the innate immune system and to elicit a synovial fluid Th17 cell response that might play a crucial role in the pathogenesis of Lyme arthritis [ABSTRACT FROM AUTHOR]

Published

2008

11. Atopy, intestinal helminth infection and total serum IgE in rural and urban adult Gambian communities.

Author

Nyan, O. A., Walraven, G. E. L., Banya, W. A. S., Milligan, P., Van Der Sande, M., Ceesay, S. M., Del Prete, G., and McAdam, K. P. W. J.

Subjects

*ALLERGIES, *INTESTINAL infections, *IMMUNOGLOBULIN E

Abstract

BackgroundThe rarity of atopy in traditional societies has been attributed to high parasite-driven blocking IgE concentrations. Information is lacking on the relationship between atopy, IgE and intestinal helminth infection in African populations. ObjectiveTo determine the prevalence of atopy and intestinal helminth infection and to relate these to wheeze history and serum total IgE in a community sample of adults from an urban (Banjul) and a rural (Farafenni) area of the Gambia. MethodsSix hundred and ninety-three adults were interviewed about respiratory symptoms using a modified version of the IUTLD questionnaire, and had skin prick testing using four allergens. Stools were examined after formol-ether concentration. Total serum IgE concentration was measured in a subset of participants. ResultsThe prevalence of atopy (mean weal diameter > = 3 mm) in the urban and rural area was 35.3% and 22.5% (P = 0.05); D. pteronyssinus and Mold mix being the common sensitizing allergens. Prevalence of wheeze in the previous 12 months was 4.4% and 3.5% for the urban and rural areas, respectively. Wheezing was not significantly associated with atopy. Seventeen per cent of urban and 8.2% of rural subjects had helminths detected in stools. There was an inverse association between atopy and intestinal helminth infection; 7% of atopic subjects had helminths, compared to 13% of non-atopic subjects (unadjusted odds ratio 0.51, 95%CI 0.24–1.1, P = 0.09; adjusted odds ratio 0.37, 95%CI 0.15–0.92, P = 0.03). Non-atopics had total serum IgE concentrations about 2.5 times the upper limit of the reference range in non-atopic Western populations. Geometric mean total serum IgE concentration was significantly higher among atopic subjects (570 IU/mL, IQR 91–833) than non-atopic subjects (259 IU/mL, IQR 274–1303) (P < 0.001). IgE concentration was not associated with the presence of helminth infection. ConclusionFurther studies are needed to clarify why... [ABSTRACT FROM AUTHOR]

Published

2001

12. Clinical effects of preemptive intra-articular lidocaine, dexmedetomidine and lidocaine-dexmedetomidine administration in dogs undergoing arthroscopy.

Author

Brioschi, F.A., Gioeni, D., Lazzarini, E., Del Prete, G., Bronzo, V., Jacchetti, A., and Carotenuto, A.M.

Subjects

*DEXMEDETOMIDINE, *LIDOCAINE, *SYSTOLIC blood pressure, *ARTHROSCOPY, *INTRA-articular injections, *DOGS

Abstract

• Intra-articular anaesthesia was useful for pain management in canine arthroscopy. • Intra-articular dexmedetomidine provided successful intraoperative analgesia. • Intraoperative analgesia using intra-articular lidocaine-dexmedetomidine was successful. • Intra-articular treatments produced similar postoperative analgesia. • Intra-articular lidocaine-dexmedetomidine promoted atrioventricular blocks in dogs. This study investigated the perioperative effects of preemptive intra-articular lidocaine (L group), dexmedetomidine (D group) and lidocaine-dexmedetomidine (LD group) in dogs. Physiological variables were intraoperatively recorded at 5 min intervals starting from baseline (5 min before intra-articular injection). If nociception occurred, IV fentanyl was administered. Postoperative pain was assessed using the Short Form-Glasgow Composite Measure Pain Scale. Twenty-four dogs (eight in each group) were included in this prospective, randomized, masked clinical study. In the LD group, systolic arterial pressure significantly increased at T10 (P = 0.027), T15 (P = 0.021) and T20 (P = 0.022), compared with baseline. In the D and LD groups, mean arterial pressure significantly increased at T10 (P = 0.022; 0.024), T15 (P = 0.024; 0.09) and T20 (P = 0.019; 0.021), compared with baseline and diastolic arterial pressure significantly increased at T10 (P = 0.026; 0.047), T15 (P = 0.021; 0.023), T20 (P = 0.011; 0.012) and T25 (P = 0.019; 0.027), compared with baseline. In the LD group, heart rate significantly decreased at T5 (P = 0.031), T10 (P = 0.026) and T15 (P = 0.034), compared with baseline. Atrioventricular blocks appeared more frequently in the LD group than in L and D groups (P = 0.002). Group L received more fentanyl than the D and LD groups (P = 0.03). No differences in postoperative pain score were detected (P = 0.121). These findings suggested systemic absorption of intra-articular dexmedetomidine. Intra-articular lidocaine-dexmedetomidine was associated with a greater incidence of atrioventricular blocks. Intra-articular dexmedetomidine, alone and combined with lidocaine, provided better intraoperative analgesia than lidocaine in dogs undergoing arthroscopy, although the 12 h postoperative analgesic effect of the three treatments was similar. [ABSTRACT FROM AUTHOR]

Published

2021

13. Abnormalities of in vitro immunoglobulin production in apparently healthy haemophiliacs: relationship with alterations of T cell subsets and with HTLV-III seropositivity.

Author

Biagiotti, R., Giudizi, M. G., Almerigogna, F., Mazzetti, M., Alessi, A., del Prete, G. F., Rafanelli, D., Fiorilli, M., Morfini, M., and Romagnani, S.

Subjects

*IMMUNOGLOBULIN G, *MITOGENS, *LECTINS, *IMMUNOGLOBULINS, *HEMAGGLUTININ, *PLASMA cells

Abstract

The pokeweed mitogen (PWM)-induced immunoglobulin (Ig) production by cultures of peripheral blood mononuclear cells (PBMC) was reduced in healthy haemophiliacs treated with commercial factor VIII (or IX) concentrate, whereas the spontaneous IgG synthesis in vitro was enhanced, PWM-induced Ig production was lower in those who had received greater amounts of concentrate, in those with inverted T4/T8 lymphocyte ratios and in those with antibody to HTLV-III, The spontaneous IgG production in vitro was higher in haemophiliacs who had received larger amounts of concentrate, in those with inverted T4/T8 ratio and in those with antibody anti-HTLV-III. However, some patients with normal T4/T8 ratio and some with HTLV-III antibody also had raised spontaneous IgG production. [ABSTRACT FROM AUTHOR]

Published

1986

14. Airway eosinophilia and expression of interleukin-5 protein in asthma and in exacerbations of chronic bronchitis.

Author

Saetta, M., di Stefano, A., Maestrelli, P., Turato, G., Mapp, C. E., Pieno, M., Zanguochi, G., del Prete, G., and Fabbri, L. M.

Subjects

*EOSINOPHILIA, *INTERLEUKIN-5, *AIRWAY (Anatomy), *ASTHMA, *BRONCHITIS, *BRONCHIAL diseases

Abstract

Background An increased number of eosinophils in the bronchial mucosa has been demonstrated both in asthma and in exacerbations of chronic bronchitis. Objective To investigate whether the airway eosinophilia present in asthma and in chronic bronchitis during exacerbations is associated with interleukin (IL)-5 protein expression in the bronchial mucosa. Methods We obtained bronchial biopsies in IS subjects with asthma (four intrinsic, seven extrinsic and seven occupational) and in 11 subjects with chronic bronchitis examined during an exacerbation. The findings were compared with those of bronchial biopsies from 10 subjects with chronic bronchitis examined tinder baseline conditions and from seven normal subjects. taken as controls. By immunohistochemistry, we assessed the expression of IL-5 protein and the number of eosinophils (FG2), mast cells (tryptase). and T-Iymphocytes (CD3) in the submucosa. Results As compared with controls, the number of eosinophills was increased to a similar degree in both asthma (P< 0.001) and in exacerbations of chronic bronchitis (P< 0.001). whereas the number of IL-5 immunopositive cells was increased significantly only in asthma (P < 0.01). No differences were observed in the number of mast cells and T-lymphocytes between the four groups of subjects examined. Conclusions This study shows that the degree of airway eosinophilia is similar in asthma and in exacerbations of chronic bronchitis. hut only in asthma is it associated with an increased expression of IL-S protein in the bronchial mucosa. [ABSTRACT FROM AUTHOR]

Published

1996