Molecular methods for the analysis of gut microbiota

Alm EW; Amann R; Amann RI; Amann RI; Anton Al; Ashelford KE; Blaut M; Bodrossy L; Bonnet R; Cousineau B; DeLong EF; El Fantroussi S; Finegold SM; Fox GE; Franks AH; Fuchs BM; Gmur R; Guschin DY; Harmsen HJ; Harmsen HJ; Harmsen HJM; Hassan AA; Hedegaard J; Heilig HG; Hodson RE; Hold GL; Hold GL; Holmstrom K; Hoshino T; Hugenholtz P; Jansen GJ; Kasai H; Lange M; Langendijk PS; Lawson PA; Lewis PJ; Loy A; Loy A; Ludwig W; Marteau P; Moore WE; Moreira D; Muyzer G; Palys T; Pemthaler J; Pemthaler J; Porter J; Poulsen LK; Rautio M; Rigottier-Gois L; Rigottier-Gois L; Rudi K; Rudi K; Saiki RK; Schwiertz A; Schwiertz A; Sghir A; Simmering R; Small J; Song Y; Steer T; Suau A; Tani K; Tani K; Tannock GW; Taras D; Taroncher-Oldenburg G; Tolker-Nielsen T; Tolker-Nielsen T; Urakawa H; Vaid A; Vaughan EE; Wallner G; Wallner G; Wallner G; Wang RF; Wang WY; Wilson KH; Woese CR; Wolin MJ; Zoetendal EG; Zoetendal EG

Molecular methods for the analysis of gut microbiota

Abstract

This review focuses on methodological approaches used to study the composition of human faecal microbiota. Gene sequencing is the most accurate tool for revealing the phylogenetic relationships between bacteria. The main application of fluorescence in situ hybridization (FISH) in both microscopy and flow cytometry is to enumerate faecal bacteria. While flow cytometry is a very fast method, FISH microscopy still has a considerably lower detection limit