PRJDB2188 C57BL/6 mice were administered with 200 microliters of PBS per os daily. After 30 days of administration, contents in small intestine from 3 mice were collected, pooled and homogenized. Genomic DNA was isolated from these intestinal contents. 16S rRNA gene fragments were then amplified using 27F and 519R primers and sequenced by barcoded-tag pyrosequencing. SAMD00009196 Group A/PBS/small intestine CTS GENOMIC PCR 0 Application Read Forward 1 454 GS FLX Titanium 1 NIL PRJDB2188 C57BL/6 mice were administered with 200 microliters of PBS per os daily. After 30 days of administration, contents in large intestine from 3 mice were collected, pooled and homogenized. Genomic DNA was isolated from these intestinal contents. 16S rRNA gene fragments were then amplified using 27F and 519R primers and sequenced by barcoded-tag pyrosequencing. SAMD00009198 Group A/PBS/small intestine CTS GENOMIC PCR 0 Application Read Forward 1 454 GS FLX Titanium 1 NIL PRJDB2188 C57BL/6 mice were administered with 2 mg PG in 200 microliters of PBS per os daily. After 30 days of administration, contents in small intestine from 3 mice were collected, pooled and homogenized. Genomic DNA was isolated from these intestinal contents. 16S rRNA gene fragments were then amplified using 27F and 519R primers and sequenced by barcoded-tag pyrosequencing. SAMD00009199 Group A/PBS/small intestine CTS GENOMIC PCR 0 Application Read Forward 1 454 GS FLX Titanium 1 NIL PRJDB2188 C57BL/6 mice were administered with 2 mg PG in 200 microliters of PBS per os daily. After 30 days of administration, contents in large intestine from 3 mice were collected, pooled and homogenized. Genomic DNA was isolated from these intestinal contents. 16S rRNA gene fragments were then amplified using 27F and 519R primers and sequenced by barcoded-tag pyrosequencing. SAMD00009193 Group A/PBS/small intestine CTS GENOMIC PCR 0 Application Read Forward 1 454 GS FLX Titanium 1 NIL PRJDB2188 C57BL/6 mice were administered with 200 microliters of PBS per os daily. After 30 days of administration, contents in small intestine from 3 mice were collected, pooled and homogenized. Genomic DNA was isolated from these intestinal contents. 16S rRNA gene fragments were then amplified using 27F and 519R primers and sequenced by barcoded-tag pyrosequencing. SAMD00009195 Group A/PBS/small intestine CTS GENOMIC PCR 0 Application Read Forward 1 454 GS FLX Titanium 1 NIL PRJDB2188 C57BL/6 mice were administered with 200 microliters of PBS per os daily. After 30 days of administration, contents in large intestine from 3 mice were collected, pooled and homogenized. Genomic DNA was isolated from these intestinal contents. 16S rRNA gene fragments were then amplified using 27F and 519R primers and sequenced by barcoded-tag pyrosequencing. SAMD00009194 Group A/PBS/small intestine CTS GENOMIC PCR 0 Application Read Forward 1 454 GS FLX Titanium 1 NIL PRJDB2188 C57BL/6 mice were administered with 2 mg PG in 200 microliters of PBS per os daily. After 30 days of administration, contents in small intestine from 3 mice were collected, pooled and homogenized. Genomic DNA was isolated from these intestinal contents. 16S rRNA gene fragments were then amplified using 27F and 519R primers and sequenced by barcoded-tag pyrosequencing. SAMD00009197 Group A/PBS/small intestine CTS GENOMIC PCR 0 Application Read Forward 1 454 GS FLX Titanium 1 NIL PRJDB2188 C57BL/6 mice were administered with 2 mg PG in 200 microliters of PBS per os daily. After 30 days of administration, contents in large intestine from 3 mice were collected, pooled and homogenized. Genomic DNA was isolated from these intestinal contents. 16S rRNA gene fragments were then amplified using 27F and 519R primers and sequenced by barcoded-tag pyrosequencing. SAMD00009200 Group A/PBS/small intestine CTS GENOMIC PCR 0 Application Read Forward 1 454 GS FLX Titanium 1 NIL