This is a test site. The production site with full data is available at GBIF.org
{{nav.loginGreeting}}
  • Get data

      • Occurrences
      • GBIF API
      • Species
      • Datasets
      • Occurrence snapshots
      • Hosted portals
      • Trends
  • How-to

    • Share data

      • Quick-start guide
      • Dataset classes
      • Data hosting
      • Standards
      • Become a publisher
      • Data quality
      • Data papers

    • Use data

      • Featured data use
      • Citation guidelines
      • GBIF citations
      • Citation widget
      • Guides and documentation
  • Tools

    • Publishing

      • IPT
      • Data validator
      • GeoPick
      • New data model
      • GRSciColl
      • Suggest a dataset
      • Metabarcoding data toolkit

    • Data access and use

      • Hosted portals
      • Scientific collections
      • Data processing
      • Derived datasets
      • rgbif
      • pygbif
      • MAXENT
      • Tools catalogue

    • GBIF labs

      • Species matching
      • Name parser
      • Sequence ID
      • Relative observation trends
      • GBIF data blog
  • Community

    • Network

      • Participant network
      • Nodes
      • Publishers
      • Network contacts
      • Community forum
      • alliance for biodiversity knowledge

    • Volunteers

      • Mentors
      • Ambassadors
      • Translators
      • Citizen scientists

    • Activities

      • Capacity development
      • Programmes & projects
      • Training and learning resources
      • Data Use Club
      • Living Atlases
  • About

    • Inside GBIF

      • What is GBIF?
      • Become a member
      • Governance
      • Strategic framework
      • Work Programme
      • Funders
      • Partnerships
      • Release notes
      • Contacts

    • News & outreach

      • News
      • Subscribe
      • Events
      • Awards
      • Science Review
      • Data use
      • Thematic communities
  • User profile

Agrobacterium LBA

Dataset
Agrobacterium-mediated gene delivery and transient expression in the red macroalga Chondrus crispus
Rank
GENUS

Classification

kingdom
Bacteria
phylum
Proteobacteria
class
Alphaproteobacteria
order
Rhizobiales
family
Rhizobiaceae
genus
Agrobacterium

description

Under the SEM, short, rod-shaped bacterial cells about 0.8 × 2 µm were seen attached in large numbers (an estimated average of one bacterial cell per µm 2) to the Chondrus thallus surface at the wound sites. Whole colonies were observed in a fibrillar mesh (Figure 2). Protocol for eliminating Agrobacterium using cefotaxime The results of testing cefotaxime concentrations of 500 and 800 mg l− 1 confirmed that this cefotaxime-supplemented wash protocol ensured that residual Agrobacterium and other culturable bacteria were eliminated on the thalli within 6 days (Table 1). Agrobacterium successfully delivered pCAMBIA 1301 into Chondrus thalli The methodology for transformation developed using pCAMBIA 1301 followed by the established wash protocol included controls to detect any false positives occurring from indigenous activity of beta-glucoronidase in Chondrus (unwounded and untransformed thalli, Figure 3 C), indigenous activity from LBA 4404 bacterial cells (pin-pricked thalli co-cultivated with untransformed Agrobacterium LBA 4404 bacteria, Figure 3 B), physiological response of algal cells to wounding (pin-pricked thalli cultivated without bacteria, Figure 3 A) and vector components (pin-pricked thalli co-cultivated with Agrobacterium LBA 4404 bearing a construct where the GUS gene is absent; pRI 910 binary vector, Figure 3 D). None of these controls were stained. However, thalli transformed with pCAMBIA 1301 were stained blue (Figure 3 E). Manipulating transformation conditions can enhance transformation efficiency As shown in Figure 4, among the pin-pricked thalli, a significant increase in transformation efficiency (higher percentage of thallus segments stained blue) was observed when seawater was used in preference to Induction Medium (Mann-Whitney test, p = 0.029) in the presence of acetosyringone. However, no transformation was detected in the unwounded thallus segments or those wounded by bombardment when co-cultivation was conducted using seawater. In addition, without the presence of acetosyringone, transformation occurred at a significantly lower efficiency of less than 10 % (Mann-Whitney, p = 0.004). Successful expression obtained with the Chondrus - specific expression cassette Using the Agrobacterium transformation protocol developed using pCAMBIA 1301, the constructed pRI 910 (Ac- GUS) was delivered into thallus cells using seawater as the co-cultivation medium and with the same controls as for pCAMBIA 1301. Blue colouration was apparent at the sites of tear, cut or wounding on Agrobacterium - mediated transformed thalli when compared to controls (Figure 5). Transverse sections through the tissue revealed blue localization of the GUS precipitate within the peripheral cortical cells and central medullary filaments. In general, a darker staining intensity was observed with pRI 910 (Ac- GUS). Furthermore, a higher transformation efficiency of 85 % was obtained with this Chondrus - specific construct as opposed to 52 % with pCAMBIA 1301.

Name

Homonyms
Agrobacterium LBA
What is GBIF? API FAQ Newsletter Privacy Terms and agreements Citation Code of Conduct Acknowledgements
Contact GBIF Secretariat Universitetsparken 15 DK-2100 Copenhagen Ø Denmark
GBIF is a Global Core Biodata Resource