Tection and amounts, was performed in 96 well detection plates in ABI prism 7000 using the Absolute Quantification protocol in 7000 SYSTEM software version 1.2.3f2 (Applied Biosystems, Stockholm, Sweden) together with standard curves ranging from 5 ng to 50 fg. Samples were analyzed in triplicates and mean CT values above 35 were considered negative to avoid detection of false positives.Materials and Methods Subjects and isolation of blood PBMCsFor this study, a total of thirty children were included from a larger prospective study cohort [21?2]. Here, children were included based on availability of fecal samples at several occasions during the first two months of life as well as availability of mononuclear cells from two years of age. All infants were healthy, born term (median weeks 40, range 38?3) and had normal birth weights (mean 3,6 kg, range 2,7?,8). Thirteen (n = 13) of the children had allergic parents and seventeen (n = 17) had nonallergic parents. The study was approved by the Human Ethics Committee at Huddinge University Hospital, Stockholm (Dnr 75/ 97, 331/02), and the parents provided informed verbal consent. No written documentation of the participants informed approval was required, which was agreed to by the Human Ethics Committee and was according to the regulations at the time of the initiation of the study. The midwife at the maternity ward asked families expecting a child if they were interested in participating in the study. If so, the pediatrician 25837696 (C.N.) in charge contacted them, gave further information and invited them to a seminar on allergies. If still interested to participate, appointments were made for blood sampling of the parents, when approval of their participation was documented. Mononuclear cells from venous blood sampled at two years of age, were separated within 24 hrs after collection, by Ficoll-Paque (Pharmacia-Upjohn, Uppsala, Sweden) gradient centrifugation. The cells were resuspended in tissue culture medium (RPMI 1640 Hepes containing 10 heat inactivated fetal calf serum and 25 mg/mL of gentamycin and 2 mm L-glutamine), supplemented with 10 MC-LR site dimethyl sulphoxide (DMSO), frozen and stored in liquid purchase SR3029 nitrogen. PBMCs from healthy adult blood donors were obtained and processed as above. All donors gave their written informed consent to participate, which was approved of by the Regional Ethics Committee in Stockholm (Dnr 04-106/1).Generation of bacterial supernatantsL. rhamnosus and S. aureus were used for the stimulation experiments: L. rhamnosus GG (ATCC 53103; isolated from the probiotic product Culturelle), and S. aureus 161.2 (producing Staphylococcal enterotoxin A and H). S. aureus strain is a kind gift ?from Asa Rosengren, The National Food Agency, Uppsala, Sweden, who also has screened the strain for toxin genes by using PCR. The lactobacilli were cultured in MRS broth (Oxoid) at 37uC for 20 h and the staphylococci in BHI broth (Merck) at 37uC for 72 h still culture. The bacteria were pelleted by centrifugation at 14 000 g where after the supernatants were sterile filtered (0,2 mm) and frozen at 220uC until used.ELISpot for quantification of cytokine secreting cells after stimulation of PBMCsBriefly, nitrocellulose plates (Millipore Corp., Bedford, MA, USA) were coated and incubated over night with anti-human monoclonal antibodies (mAbs) to IL-4, IL-10 and IFN-c (Mabtech, Nacka, Sweden), at a concentration of 10 mg/ml, as described in detail elsewhere [23]. Cells were thawed and washedIn vit.Tection and amounts, was performed in 96 well detection plates in ABI prism 7000 using the Absolute Quantification protocol in 7000 SYSTEM software version 1.2.3f2 (Applied Biosystems, Stockholm, Sweden) together with standard curves ranging from 5 ng to 50 fg. Samples were analyzed in triplicates and mean CT values above 35 were considered negative to avoid detection of false positives.Materials and Methods Subjects and isolation of blood PBMCsFor this study, a total of thirty children were included from a larger prospective study cohort [21?2]. Here, children were included based on availability of fecal samples at several occasions during the first two months of life as well as availability of mononuclear cells from two years of age. All infants were healthy, born term (median weeks 40, range 38?3) and had normal birth weights (mean 3,6 kg, range 2,7?,8). Thirteen (n = 13) of the children had allergic parents and seventeen (n = 17) had nonallergic parents. The study was approved by the Human Ethics Committee at Huddinge University Hospital, Stockholm (Dnr 75/ 97, 331/02), and the parents provided informed verbal consent. No written documentation of the participants informed approval was required, which was agreed to by the Human Ethics Committee and was according to the regulations at the time of the initiation of the study. The midwife at the maternity ward asked families expecting a child if they were interested in participating in the study. If so, the pediatrician 25837696 (C.N.) in charge contacted them, gave further information and invited them to a seminar on allergies. If still interested to participate, appointments were made for blood sampling of the parents, when approval of their participation was documented. Mononuclear cells from venous blood sampled at two years of age, were separated within 24 hrs after collection, by Ficoll-Paque (Pharmacia-Upjohn, Uppsala, Sweden) gradient centrifugation. The cells were resuspended in tissue culture medium (RPMI 1640 Hepes containing 10 heat inactivated fetal calf serum and 25 mg/mL of gentamycin and 2 mm L-glutamine), supplemented with 10 dimethyl sulphoxide (DMSO), frozen and stored in liquid nitrogen. PBMCs from healthy adult blood donors were obtained and processed as above. All donors gave their written informed consent to participate, which was approved of by the Regional Ethics Committee in Stockholm (Dnr 04-106/1).Generation of bacterial supernatantsL. rhamnosus and S. aureus were used for the stimulation experiments: L. rhamnosus GG (ATCC 53103; isolated from the probiotic product Culturelle), and S. aureus 161.2 (producing Staphylococcal enterotoxin A and H). S. aureus strain is a kind gift ?from Asa Rosengren, The National Food Agency, Uppsala, Sweden, who also has screened the strain for toxin genes by using PCR. The lactobacilli were cultured in MRS broth (Oxoid) at 37uC for 20 h and the staphylococci in BHI broth (Merck) at 37uC for 72 h still culture. The bacteria were pelleted by centrifugation at 14 000 g where after the supernatants were sterile filtered (0,2 mm) and frozen at 220uC until used.ELISpot for quantification of cytokine secreting cells after stimulation of PBMCsBriefly, nitrocellulose plates (Millipore Corp., Bedford, MA, USA) were coated and incubated over night with anti-human monoclonal antibodies (mAbs) to IL-4, IL-10 and IFN-c (Mabtech, Nacka, Sweden), at a concentration of 10 mg/ml, as described in detail elsewhere [23]. Cells were thawed and washedIn vit.