16S rRNA-Based Analysis of Microbiota from the Cecum of Broiler Chickens

doi:10.1128/AEM.68.1.124-137.2002

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Applied and Environmental Microbiology, January 2002, p. 124-137, Vol. 68, No. 1
0099-2240/02/$04.00+0 DOI: 10.1128/AEM.68.1.124-137.2002
Copyright © 2002, American Society for Microbiology. All Rights Reserved.

16S rRNA-Based Analysis of Microbiota from the Cecum of Broiler Chickens

Xiang Y. Zhu, Tanya Zhong, Yoga Pandya, and Rolf D. Joerger^*

Department of Animal and Food Sciences, University of Delaware, Newark, Delaware 19717-1301

Received 26 July 2001/ Accepted 12 October 2001

The microbiota of the intestinal tract of chickens plays animportant role in inhibiting the establishment of intestinalpathogens. Earlier culturing and microscopic examinations indicatedthat only a fraction of the bacteria in the cecum of chickenscould be grown in the laboratory. Therefore, a survey of cecalbacteria was done by retrieval of 16S rRNA gene sequences fromDNA isolated from the cecal content and the cecal mucosa. Theribosomal gene sequences were amplified with universal primersand cloned or subjected to temporal temperature gradient gelelectrophoresis (TTGE). Partial 16S rRNA gene sequences weredetermined from the clones and from the major bands in TTGEgels. A total of 1,656 partial 16S rRNA gene sequences wereobtained and compared to sequences in the GenBank. The comparisonindicated that 243 different sequences were present in the samples.Overall, sequences representing 50 phylogenetic groups or subgroupsof bacteria were found, but approximately 89% of the sequencesrepresented just four phylogenetic groups (Clostridium leptum,Sporomusa sp., Clostridium coccoides, and enterics). Sequencesof members of the Bacteroides group, the Bifidobacterium infantissubgroup, and of Pseudomonas sp. each accounted for less than2% of the total. Sequences related to those from the Escherichiasp. subgroup and from Lactobacillus, Pseudomonas, and Bifidobacteriumspp. were generally between 98 and 100% identical to sequencesalready deposited in the GenBank. Sequences most closely relatedto those of the other bacteria were generally 97% or less identicalto those in the databases and therefore might be from currentlyunknown species. TTGE and random cloning indicated that certainphylogenetic subgroups were common to all birds analyzed, butsequence data from random cloning also provided evidence forqualitative and quantitative differences among the cecal microbiotaof individual birds reared under very similar conditions.

* Corresponding author. Mailing address: Department of Animal and Food Sciences, University of Delaware, 018 Townsend Hall, Newark, DE 19717-1303. Phone: (302) 831-6605. Fax: (302) 831-2822. Email: rjoerger{at}udel.edu.

Published as paper no. 1700 in the Journal Series of the DelawareAgricultural Experiment Station.

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