Safranine fluorescent staining of wood cell walls.
Identifieur interne : 003823 ( Main/Exploration ); précédent : 003822; suivant : 003824Safranine fluorescent staining of wood cell walls.
Auteurs : J. Bond [Nouvelle-Zélande] ; L. Donaldson ; S. Hill ; K. HitchcockSource :
- Biotechnic & histochemistry : official publication of the Biological Stain Commission [ 1473-7760 ] ; 2008.
Descripteurs français
- KwdFr :
- Bois (composition chimique), Bois (cytologie), Colorants fluorescents (MeSH), Coloration et marquage (MeSH), Lignine (composition chimique), Paroi cellulaire (composition chimique), Phénazines (MeSH), Pinus (composition chimique), Pinus (cytologie), Populus (composition chimique), Populus (cytologie), Pseudotsuga (composition chimique), Pseudotsuga (cytologie).
- MESH :
- composition chimique : Bois, Lignine, Paroi cellulaire, Pinus, Populus, Pseudotsuga.
- cytologie : Bois, Pinus, Populus, Pseudotsuga.
- Colorants fluorescents, Coloration et marquage, Phénazines.
English descriptors
- KwdEn :
- MESH :
- chemical , chemistry : Lignin.
- chemical : Fluorescent Dyes, Phenazines.
- chemistry : Cell Wall, Pinus, Populus, Pseudotsuga, Wood.
- cytology : Pinus, Populus, Pseudotsuga, Wood.
- Staining and Labeling.
Abstract
Safranine is an azo dye commonly used for plant microscopy, especially as a stain for lignified tissues such as xylem. Safranine fluorescently labels the wood cell wall, producing green/yellow fluorescence in the secondary cell wall and red/orange fluorescence in the middle lamella (ML) region. We examined the fluorescence behavior of safranine under blue light excitation using a variety of wood- and fiber-based samples of known composition to interpret the observed color differentiation of different cell wall types. We also examined the basis for the differences in fluorescence emission using spectral confocal microscopy to examine lignin-rich and cellulose-rich cell walls including reaction wood and decayed wood compared to normal wood. Our results indicate that lignin-rich cell walls, such as the ML of tracheids, the secondary wall of compression wood tracheids, and wood decayed by brown rot, tend to fluoresce red or orange, while cellulose-rich cell walls such as resin canals, wood decayed by white rot, cotton fibers and the G-layer of tension wood fibers, tend to fluoresce green/yellow. This variation in fluorescence emission seems to be due to factors including an emission shift toward red wavelengths combined with dye quenching at shorter wavelengths in regions with high lignin content. Safranine fluorescence provides a useful way to differentiate lignin-rich and cellulose-rich cell walls without counterstaining as required for bright field microscopy.
DOI: 10.1080/10520290802373354
PubMed: 18802812
Affiliations:
Links toward previous steps (curation, corpus...)
Le document en format XML
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Hitchcock</name></author></titleStmt><publicationStmt><idno type="wicri:source">PubMed</idno><date when="2008">2008</date><idno type="RBID">pubmed:18802812</idno><idno type="pmid">18802812</idno><idno type="doi">10.1080/10520290802373354</idno><idno type="wicri:Area/Main/Corpus">003793</idno><idno type="wicri:explorRef" wicri:stream="Main" wicri:step="Corpus" wicri:corpus="PubMed">003793</idno><idno type="wicri:Area/Main/Curation">003793</idno><idno type="wicri:explorRef" wicri:stream="Main" wicri:step="Curation">003793</idno><idno type="wicri:Area/Main/Exploration">003793</idno></publicationStmt><sourceDesc><biblStruct><analytic><title xml:lang="en">Safranine fluorescent staining of wood cell walls.</title><author><name sortKey="Bond, J" sort="Bond, J" uniqKey="Bond J" first="J" last="Bond">J. Bond</name><affiliation wicri:level="1"><nlm:affiliation>Cellwall Biotechnology Centre, Rotorua, New Zealand. Suprajac@yahoo.com</nlm:affiliation><country xml:lang="fr">Nouvelle-Zélande</country><wicri:regionArea>Cellwall Biotechnology Centre, Rotorua</wicri:regionArea><wicri:noRegion>Rotorua</wicri:noRegion></affiliation></author><author><name sortKey="Donaldson, L" sort="Donaldson, L" uniqKey="Donaldson L" first="L" last="Donaldson">L. Donaldson</name></author><author><name sortKey="Hill, S" sort="Hill, S" uniqKey="Hill S" first="S" last="Hill">S. Hill</name></author><author><name sortKey="Hitchcock, K" sort="Hitchcock, K" uniqKey="Hitchcock K" first="K" last="Hitchcock">K. Hitchcock</name></author></analytic><series><title level="j">Biotechnic & histochemistry : official publication of the Biological Stain Commission</title><idno type="eISSN">1473-7760</idno><imprint><date when="2008" type="published">2008</date></imprint></series></biblStruct></sourceDesc></fileDesc><profileDesc><textClass><keywords scheme="KwdEn" xml:lang="en"><term>Cell Wall (chemistry)</term><term>Fluorescent Dyes (MeSH)</term><term>Lignin (chemistry)</term><term>Phenazines (MeSH)</term><term>Pinus (chemistry)</term><term>Pinus (cytology)</term><term>Populus (chemistry)</term><term>Populus (cytology)</term><term>Pseudotsuga (chemistry)</term><term>Pseudotsuga (cytology)</term><term>Staining and Labeling (MeSH)</term><term>Wood (chemistry)</term><term>Wood (cytology)</term></keywords><keywords scheme="KwdFr" xml:lang="fr"><term>Bois (composition chimique)</term><term>Bois (cytologie)</term><term>Colorants fluorescents (MeSH)</term><term>Coloration et marquage (MeSH)</term><term>Lignine (composition chimique)</term><term>Paroi cellulaire (composition chimique)</term><term>Phénazines (MeSH)</term><term>Pinus (composition chimique)</term><term>Pinus (cytologie)</term><term>Populus (composition chimique)</term><term>Populus (cytologie)</term><term>Pseudotsuga (composition chimique)</term><term>Pseudotsuga (cytologie)</term></keywords><keywords scheme="MESH" type="chemical" qualifier="chemistry" xml:lang="en"><term>Lignin</term></keywords><keywords scheme="MESH" type="chemical" xml:lang="en"><term>Fluorescent Dyes</term><term>Phenazines</term></keywords><keywords scheme="MESH" qualifier="chemistry" xml:lang="en"><term>Cell Wall</term><term>Pinus</term><term>Populus</term><term>Pseudotsuga</term><term>Wood</term></keywords><keywords scheme="MESH" qualifier="composition chimique" xml:lang="fr"><term>Bois</term><term>Lignine</term><term>Paroi cellulaire</term><term>Pinus</term><term>Populus</term><term>Pseudotsuga</term></keywords><keywords scheme="MESH" qualifier="cytologie" xml:lang="fr"><term>Bois</term><term>Pinus</term><term>Populus</term><term>Pseudotsuga</term></keywords><keywords scheme="MESH" qualifier="cytology" xml:lang="en"><term>Pinus</term><term>Populus</term><term>Pseudotsuga</term><term>Wood</term></keywords><keywords scheme="MESH" xml:lang="en"><term>Staining and Labeling</term></keywords><keywords scheme="MESH" xml:lang="fr"><term>Colorants fluorescents</term><term>Coloration et marquage</term><term>Phénazines</term></keywords></textClass></profileDesc></teiHeader><front><div type="abstract" xml:lang="en">Safranine is an azo dye commonly used for plant microscopy, especially as a stain for lignified tissues such as xylem. Safranine fluorescently labels the wood cell wall, producing green/yellow fluorescence in the secondary cell wall and red/orange fluorescence in the middle lamella (ML) region. We examined the fluorescence behavior of safranine under blue light excitation using a variety of wood- and fiber-based samples of known composition to interpret the observed color differentiation of different cell wall types. We also examined the basis for the differences in fluorescence emission using spectral confocal microscopy to examine lignin-rich and cellulose-rich cell walls including reaction wood and decayed wood compared to normal wood. Our results indicate that lignin-rich cell walls, such as the ML of tracheids, the secondary wall of compression wood tracheids, and wood decayed by brown rot, tend to fluoresce red or orange, while cellulose-rich cell walls such as resin canals, wood decayed by white rot, cotton fibers and the G-layer of tension wood fibers, tend to fluoresce green/yellow. This variation in fluorescence emission seems to be due to factors including an emission shift toward red wavelengths combined with dye quenching at shorter wavelengths in regions with high lignin content. Safranine fluorescence provides a useful way to differentiate lignin-rich and cellulose-rich cell walls without counterstaining as required for bright field microscopy.</div></front></TEI><pubmed><MedlineCitation Status="MEDLINE" Owner="NLM"><PMID Version="1">18802812</PMID><DateCompleted><Year>2009</Year><Month>09</Month><Day>29</Day></DateCompleted><DateRevised><Year>2014</Year><Month>03</Month><Day>31</Day></DateRevised><Article PubModel="Print"><Journal><ISSN IssnType="Electronic">1473-7760</ISSN><JournalIssue CitedMedium="Internet"><Volume>83</Volume><Issue>3-4</Issue><PubDate><Year>2008</Year><Month>Jun</Month></PubDate></JournalIssue><Title>Biotechnic & histochemistry : official publication of the Biological Stain Commission</Title><ISOAbbreviation>Biotech Histochem</ISOAbbreviation></Journal><ArticleTitle>Safranine fluorescent staining of wood cell walls.</ArticleTitle><Pagination><MedlinePgn>161-71</MedlinePgn></Pagination><ELocationID EIdType="doi" ValidYN="Y">10.1080/10520290802373354</ELocationID><Abstract><AbstractText>Safranine is an azo dye commonly used for plant microscopy, especially as a stain for lignified tissues such as xylem. Safranine fluorescently labels the wood cell wall, producing green/yellow fluorescence in the secondary cell wall and red/orange fluorescence in the middle lamella (ML) region. We examined the fluorescence behavior of safranine under blue light excitation using a variety of wood- and fiber-based samples of known composition to interpret the observed color differentiation of different cell wall types. We also examined the basis for the differences in fluorescence emission using spectral confocal microscopy to examine lignin-rich and cellulose-rich cell walls including reaction wood and decayed wood compared to normal wood. Our results indicate that lignin-rich cell walls, such as the ML of tracheids, the secondary wall of compression wood tracheids, and wood decayed by brown rot, tend to fluoresce red or orange, while cellulose-rich cell walls such as resin canals, wood decayed by white rot, cotton fibers and the G-layer of tension wood fibers, tend to fluoresce green/yellow. This variation in fluorescence emission seems to be due to factors including an emission shift toward red wavelengths combined with dye quenching at shorter wavelengths in regions with high lignin content. Safranine fluorescence provides a useful way to differentiate lignin-rich and cellulose-rich cell walls without counterstaining as required for bright field microscopy.</AbstractText></Abstract><AuthorList CompleteYN="Y"><Author ValidYN="Y"><LastName>Bond</LastName><ForeName>J</ForeName><Initials>J</Initials><AffiliationInfo><Affiliation>Cellwall Biotechnology Centre, Rotorua, New Zealand. Suprajac@yahoo.com</Affiliation></AffiliationInfo></Author><Author ValidYN="Y"><LastName>Donaldson</LastName><ForeName>L</ForeName><Initials>L</Initials></Author><Author ValidYN="Y"><LastName>Hill</LastName><ForeName>S</ForeName><Initials>S</Initials></Author><Author ValidYN="Y"><LastName>Hitchcock</LastName><ForeName>K</ForeName><Initials>K</Initials></Author></AuthorList><Language>eng</Language><PublicationTypeList><PublicationType UI="D003160">Comparative Study</PublicationType><PublicationType UI="D016428">Journal Article</PublicationType></PublicationTypeList></Article><MedlineJournalInfo><Country>England</Country><MedlineTA>Biotech Histochem</MedlineTA><NlmUniqueID>9107378</NlmUniqueID><ISSNLinking>1052-0295</ISSNLinking></MedlineJournalInfo><ChemicalList><Chemical><RegistryNumber>0</RegistryNumber><NameOfSubstance UI="D005456">Fluorescent Dyes</NameOfSubstance></Chemical><Chemical><RegistryNumber>0</RegistryNumber><NameOfSubstance UI="D010619">Phenazines</NameOfSubstance></Chemical><Chemical><RegistryNumber>9005-53-2</RegistryNumber><NameOfSubstance UI="D008031">Lignin</NameOfSubstance></Chemical><Chemical><RegistryNumber>XTX0YXU2HV</RegistryNumber><NameOfSubstance UI="C009195">safranine T</NameOfSubstance></Chemical></ChemicalList><CitationSubset>IM</CitationSubset><MeshHeadingList><MeshHeading><DescriptorName UI="D002473" MajorTopicYN="N">Cell Wall</DescriptorName><QualifierName UI="Q000737" MajorTopicYN="Y">chemistry</QualifierName></MeshHeading><MeshHeading><DescriptorName UI="D005456" MajorTopicYN="Y">Fluorescent Dyes</DescriptorName></MeshHeading><MeshHeading><DescriptorName UI="D008031" MajorTopicYN="N">Lignin</DescriptorName><QualifierName UI="Q000737" MajorTopicYN="N">chemistry</QualifierName></MeshHeading><MeshHeading><DescriptorName UI="D010619" MajorTopicYN="Y">Phenazines</DescriptorName></MeshHeading><MeshHeading><DescriptorName UI="D028223" MajorTopicYN="N">Pinus</DescriptorName><QualifierName UI="Q000737" MajorTopicYN="N">chemistry</QualifierName><QualifierName UI="Q000166" MajorTopicYN="N">cytology</QualifierName></MeshHeading><MeshHeading><DescriptorName UI="D032107" MajorTopicYN="N">Populus</DescriptorName><QualifierName UI="Q000737" MajorTopicYN="N">chemistry</QualifierName><QualifierName UI="Q000166" MajorTopicYN="N">cytology</QualifierName></MeshHeading><MeshHeading><DescriptorName UI="D028224" MajorTopicYN="N">Pseudotsuga</DescriptorName><QualifierName UI="Q000737" MajorTopicYN="N">chemistry</QualifierName><QualifierName UI="Q000166" MajorTopicYN="N">cytology</QualifierName></MeshHeading><MeshHeading><DescriptorName UI="D013194" MajorTopicYN="Y">Staining and Labeling</DescriptorName></MeshHeading><MeshHeading><DescriptorName UI="D014934" MajorTopicYN="N">Wood</DescriptorName><QualifierName UI="Q000737" MajorTopicYN="Y">chemistry</QualifierName><QualifierName UI="Q000166" MajorTopicYN="Y">cytology</QualifierName></MeshHeading></MeshHeadingList></MedlineCitation><PubmedData><History><PubMedPubDate PubStatus="pubmed"><Year>2008</Year><Month>9</Month><Day>20</Day><Hour>9</Hour><Minute>0</Minute></PubMedPubDate><PubMedPubDate PubStatus="medline"><Year>2009</Year><Month>9</Month><Day>30</Day><Hour>6</Hour><Minute>0</Minute></PubMedPubDate><PubMedPubDate PubStatus="entrez"><Year>2008</Year><Month>9</Month><Day>20</Day><Hour>9</Hour><Minute>0</Minute></PubMedPubDate></History><PublicationStatus>ppublish</PublicationStatus><ArticleIdList><ArticleId IdType="pubmed">18802812</ArticleId><ArticleId IdType="pii">902566396</ArticleId><ArticleId IdType="doi">10.1080/10520290802373354</ArticleId></ArticleIdList></PubmedData></pubmed><affiliations><list><country><li>Nouvelle-Zélande</li></country></list><tree><noCountry><name sortKey="Donaldson, L" sort="Donaldson, L" uniqKey="Donaldson L" first="L" last="Donaldson">L. Donaldson</name><name sortKey="Hill, S" sort="Hill, S" uniqKey="Hill S" first="S" last="Hill">S. Hill</name><name sortKey="Hitchcock, K" sort="Hitchcock, K" uniqKey="Hitchcock K" first="K" last="Hitchcock">K. Hitchcock</name></noCountry><country name="Nouvelle-Zélande"><noRegion><name sortKey="Bond, J" sort="Bond, J" uniqKey="Bond J" first="J" last="Bond">J. Bond</name></noRegion></country></tree></affiliations></record>Pour manipuler ce document sous Unix (Dilib)
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