A SHORTENED RNA-FISH PROTOCOL FOR ANALYZING ARTWORKS’ MICROCOLONIZERS

dc.contributor.authorGonzález-Pérez, Marina
dc.contributor.authorde Oliveira Baptista, Sara Margarida
dc.contributor.authorPereira, António
dc.contributor.authorCandeias, António
dc.contributor.authorCaldeira, Ana Teresa
dc.date.accessioned2017-01-19T16:34:26Z
dc.date.available2017-01-19T16:34:26Z
dc.date.issued2017-01-04
dc.description.abstractMicroorganisms are involved in the deterioration of Cultural Heritage. Thus, there is a need to enhance the techniques used for their detection and identification. RNA Fluorescent In Situ Hybridization (RNA-FISH) has been successfully applied for phylogenetic identification of the viable components of the microbial communities colonizing artworks both in situ and ex situ. Until recently, it was time-consuming, taking not less than 6 h for the analysis. We have developed an RNA-FISH in suspension protocol that allowed ex situ analysis of microorganisms involved in artworks’ biodeterioration in 5 h. In this work, three modified protocols, involving microwave heating, were evaluated for further shortening two of the four main critical steps in RNA-FISH: hybridization and washing. The original and modified protocols were applied in cellular suspensions of bacteria and yeast isolates. The results obtained were evaluated and compared in terms of detectability and specificity of the signals detected by epifluorescence microscopy. One of the methods tested showed good and specific FISH signals for all the microorganisms selected and did not produce signals evidencing non-specific or fixation-induced fluorescence. This 3 h protocol allows a remarkable reduction of the time usually required for performing RNA-FISH analysis in Cultural Heritage samples. Thus, a rapid alternative for analyzing yeast and bacteria cells colonizing artworks’ surfaces by RNA-FISH is presented in this work.por
dc.identifier.authoremailmarinagp@uevora.pt
dc.identifier.authoremailsara.margot.31@gmail.com
dc.identifier.authoremailamlp@uevora.pt
dc.identifier.authoremailcandeias@uevora.pt
dc.identifier.authoremailatc@uevora.pt
dc.identifier.citationGonzález-Pérez, M; de Oliveira Baptista, S.M.; Pereira, A; Candeias, A.; Caldeira, A.T.; A shortened RNA-FISH protocol for analyzing artworks' microcolonizers.Istanbul International Conference On Progress In Applied Science 2017 (ICPAS 2017), p. 136-140. ISBN 978-605-9546-02-7. Istambul, Turkey, January 4-6, 2017.por
dc.identifier.isbn978-605-9546-02-7
dc.identifier.scientificarea365por
dc.identifier.urihttp://hdl.handle.net/10174/19896
dc.language.isoengpor
dc.peerreviewedyespor
dc.publisherYILDIZ TECHNICAL UNIVERSITY’S TECHNOPARK COMPANY OF PROMECH TEKNOLOJİ VE BİLİŞİM SİSTEMLERİ SANAYİ LTD. ŞTİ.por
dc.rightsopenAccesspor
dc.subjectFluorescence In Situ Hybridizationpor
dc.subjectMicroorganismspor
dc.subjectBiodeteriorationpor
dc.subjectCultural Heritagepor
dc.titleA SHORTENED RNA-FISH PROTOCOL FOR ANALYZING ARTWORKS’ MICROCOLONIZERSpor
dc.typearticlepor
rcaap.description.embargofctThis work was co- financed by FCT – Fundação para a Ciência e a Tecnologia through the project "MICROTECHART- Microorganisms Thriving on and Endamaging Cultural Heritage -an Analytical Rapid Tool-" (PTDC/BBBIMG/ 0046/2014) and by European Union, European Regional Development Fund ALENTEJO 2020 through the project “HIT3CH - HERCULES Interface for Technology Transfer and Teaming in Cultural Heritage” (ALT20-03-0246-FEDER-000004). Marina González-Pérez acknowledges FCT for the economic support through the post-doctoral grant SFRH/BPD/100754/2014.;

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