On through stimulating gut-associated lymphoid tissu (GALT) functions and intestinal IgA

On through stimulating gut-associated lymphoid tissu (GALT) functions and intestinal IgA

On through stimulating gut-associated lymphoid tissu (GALT) functions and intestinal IgA response after E. coli K88 challenge in piglets.Table 1. Ingredient and chemical composition of the milkreplacer formula1.Component Crude Protein Energy MJ/kg2 Lactose Calcium Total PhosphorusMilk-replacer 25.86 20.28 34.80 0.95 0.Materials and Methods Animals and Experimental DesignTwenty-eight 4-day-old male Landrace6Large White piglets were obtained from by a commercial pig farm and transported to the Laboratory of Animal Metabolism at China Agricultural University (Beijing, China). All procedures of this experiment complied with the animal care protocol which was approved by the China Agricultural University Animal Care and Use Committee. And China Agricultural University Animal Care and Use Committee specifically approved this study. NCG was purchased from Sigma-Aldrich Corporate (Louis, Missouri, US). The piglets were assigned into 11967625 four groups in a randomized complete block design according to their Contributes to cancer pathogenesis in adult animals [1]. Once transcription has been initial body weight: sham challenge (I), sham challenge + NCG (II), E. coli challenge (III), E. coli challenge + NCG (IV). Diets in group II and group IV were supplemented with 50 mg/kg body weight NCG added in Milkreplacer formula. E. coli was administered as a pathogen to establish the model of intestinal inflammation. Piglets were housed in individual metabolic cages (0.7 m61.7 m) in a temperature controlled nursery room (32?4uC for the first week, 30?2uC for the second week ). 1315463 Two sham challenge groups and two E. coli K88 challenge groups were housed in two separate nursery rooms. The composition and nutrient levels of the milk-replacer formula are shown in Table 1. The Milk-replacer formula was diluted to onefifth of its concentration with drinking water on the basis of dry material concentration of sow’s milk. All the piglets were artificially fed every 4 hours using nursing bottles. Meanwhile, metal sheet were put under the nursing cages in order to collect the formula waste; therefore, the K162 cost intake of formula was recorded accurately. On d 8, all the piglets were weighed again. Piglets in the E. coli challenged groups were orally administrated with 5 mL E. coli K88 (108 CFU/mL, purchased from the Chinese Academy of Sciences), the dose was provided by using a 10 cm tube attached on a syringe based on the results of our preliminary experiment; piglets in sham challenge groups, however, were administrated on equal volume of drinking water. The culture of E. coli K88 was grown for 20 h in a Luria broth at 37uC using 0.1 mL of inoculum from stock. Then, cells were washed twice using PBS. Next, the culture was centrifuged for 15 min at 3,0006g. Supernatants were discarded and cells were re-suspended in PBS at concentration of 108 CFU/mL of E. coli K88 (calculated based on the optical density established by serial dilution before viable bacterial count), which was directly used for the oral challenge to piglets. On day 13, all the piglets were weighed and euthanized after overnight fast. Jugular venous blood samples from each piglet (5 mL) were obtained 4 h after the last meal. The blood samples were centrifuged for 10 min at 3,0006g to obtain serum samples, which were immediately stored at 220uC until sample analysis. A 15 cm section of each intestinal segment (at the middle location), including duodenum, jejunum and ileum, was flushed gently withThe analyzed contents of amino acids in diets Essential Threoline Valine Isoleucine Leucine Phen.On through stimulating gut-associated lymphoid tissu (GALT) functions and intestinal IgA response after E. coli K88 challenge in piglets.Table 1. Ingredient and chemical composition of the milkreplacer formula1.Component Crude Protein Energy MJ/kg2 Lactose Calcium Total PhosphorusMilk-replacer 25.86 20.28 34.80 0.95 0.Materials and Methods Animals and Experimental DesignTwenty-eight 4-day-old male Landrace6Large White piglets were obtained from by a commercial pig farm and transported to the Laboratory of Animal Metabolism at China Agricultural University (Beijing, China). All procedures of this experiment complied with the animal care protocol which was approved by the China Agricultural University Animal Care and Use Committee. And China Agricultural University Animal Care and Use Committee specifically approved this study. NCG was purchased from Sigma-Aldrich Corporate (Louis, Missouri, US). The piglets were assigned into 11967625 four groups in a randomized complete block design according to their initial body weight: sham challenge (I), sham challenge + NCG (II), E. coli challenge (III), E. coli challenge + NCG (IV). Diets in group II and group IV were supplemented with 50 mg/kg body weight NCG added in Milkreplacer formula. E. coli was administered as a pathogen to establish the model of intestinal inflammation. Piglets were housed in individual metabolic cages (0.7 m61.7 m) in a temperature controlled nursery room (32?4uC for the first week, 30?2uC for the second week ). 1315463 Two sham challenge groups and two E. coli K88 challenge groups were housed in two separate nursery rooms. The composition and nutrient levels of the milk-replacer formula are shown in Table 1. The Milk-replacer formula was diluted to onefifth of its concentration with drinking water on the basis of dry material concentration of sow’s milk. All the piglets were artificially fed every 4 hours using nursing bottles. Meanwhile, metal sheet were put under the nursing cages in order to collect the formula waste; therefore, the intake of formula was recorded accurately. On d 8, all the piglets were weighed again. Piglets in the E. coli challenged groups were orally administrated with 5 mL E. coli K88 (108 CFU/mL, purchased from the Chinese Academy of Sciences), the dose was provided by using a 10 cm tube attached on a syringe based on the results of our preliminary experiment; piglets in sham challenge groups, however, were administrated on equal volume of drinking water. The culture of E. coli K88 was grown for 20 h in a Luria broth at 37uC using 0.1 mL of inoculum from stock. Then, cells were washed twice using PBS. Next, the culture was centrifuged for 15 min at 3,0006g. Supernatants were discarded and cells were re-suspended in PBS at concentration of 108 CFU/mL of E. coli K88 (calculated based on the optical density established by serial dilution before viable bacterial count), which was directly used for the oral challenge to piglets. On day 13, all the piglets were weighed and euthanized after overnight fast. Jugular venous blood samples from each piglet (5 mL) were obtained 4 h after the last meal. The blood samples were centrifuged for 10 min at 3,0006g to obtain serum samples, which were immediately stored at 220uC until sample analysis. A 15 cm section of each intestinal segment (at the middle location), including duodenum, jejunum and ileum, was flushed gently withThe analyzed contents of amino acids in diets Essential Threoline Valine Isoleucine Leucine Phen.

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