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Expansion microscopy applied to mono- and dual-species biofilms
被引:0
|作者:
David Valdivieso González
Josué Jara
Víctor G. Almendro-Vedia
Belén Orgaz
Iván López-Montero
机构:
[1] Universidad Complutense de Madrid,Dto. Química Física
[2] Avda. Complutense s/n,Instituto Pluridisciplinar
[3] Universidad Complutense de Madrid,Sección Departamental de Nutrición y Ciencia de los Alimentos, Facultad de Veterinaria
[4] Ps. Juan XXIII 1,Sección Departamental de Farmacia Galénica y Tecnología Alimentaria, Facultad de Veterinaria
[5] Instituto de Investigación Biomédica Hospital Doce de Octubre (Imas12),undefined
[6] Avda. de Córdoba s/n,undefined
[7] Universidad Complutense de Madrid,undefined
[8] Universidad Complutense de Madrid,undefined
[9] Avda. Complutense s/n,undefined
[10] Instituto de Investigación Biomédica Hospital Doce de Octubre (Imas12),undefined
[11] Avda. de Córdoba s/n,undefined
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摘要:
Expansion microscopy (ExM) is a new super-resolution technique based on embedding the biological sample within a hydrogel and its physical expansion after swelling. This allows increasing its size by several times while preserving its structural details. Applied to prokaryotic cells, ExM requires digestion steps for efficient expansion as bacteria are surrounded by a rigid cell wall. Furthermore, bacteria can live in social groups forming biofilms, where cells are protected from environmental stresses by a self-produced matrix. The extracellular matrix represents an additional impenetrable barrier for ExM. Here we optimize the current protocols of ExM and apply them to mono- and dual-species biofilms formed by clinical isolates of Limosilactobacillus reuteri, Enterococcus faecalis, Serratia marcescens and Staphylococcus aureus. Using scanning electron microscopy for comparison, our results demonstrate that embedded bacteria expanded 3-fold. Moreover, ExM allowed visualizing the three-dimensional architecture of the biofilm and identifying the distribution of different microbial species and their interactions. We also detected the presence of the extracellular matrix after expansion with a specific stain of the polysaccharide component. The potential applications of ExM in biofilms will improve our understanding of these complex communities and have far-reaching implications for industrial and clinical research.
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