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Sequence data for plasmids developed by the Baulcombe group including virus vectors and suppressors of RNA silencing

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https://www.repository.cam.ac.uk/handle/1810/376159

Repository DOI

https://doi.org/10.17863/CAM.113511
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protocols.zip (408.98 KB)

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Method

Change log

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Description

The sequences and maps of the Chlamydomonas artificial miRNA vectors pChlamiRNA2, pChlamyRNA3 and pChlamyRNA3int

  • pChlamiRNA2 (gb file)
  • pChlamiRNA2_map (jpg)
  • pChlamiRNA2_sequence (txt)
  • pChlamiRNA3 (gb)
  • pChlamiRNA3_map (jpg)
  • pChlamiRNA3_sequence (txt)
  • pChlamiRNA3int (gb)
  • pChlamiRNA3int_map (jpg)
  • pChlamiRNA3int_sequence (txt)

PVX vectors

  • pGR106 (Vector NTI)
  • pGR106 (Sequence, Word format)
  • pGR106 diagram (Powerpoint format)
  • pGR106 polylinker seq (Word)
  • pGR107 polylinker seq (Word)

TRV vectors

  • pTV00.doc
  • pBINTRA6.doc

Suppressors of Gene Silencing

Constructing pBin61:
The 35Spro-35Ster expression cassette of pJIT61 was excised as a kpnI-XhoI fragment and mobilised into the pBin19 binary vector T-DNA. The cassette was inserted into KpnI-SalI digested pBin19, therefore eliminating the SalI site. This led to plasmid pBin61. You will find the sequence of the vector as a MS Word file.

Inserting suppressors of gene silencing into pBin61:
The SmaI site in pBin61 was used to clone all the viral suppressors in sense orientation. Blunt-end PCR-amplified fragments of the suppressors were used for cloning. It is therefore not possible to excise the suppressor sequence from the pBin61 vector. You will find sequences of each individual suppressor constructs cloned in pBin61.

  • pBIN61-2b.doc
  • pBIN61-AC2.doc
  • pBIN61-HcPro.doc
  • pBIN61-P1.doc
  • pBIN61-P19.doc
  • pBIN61-P25.doc
  • pBin61.doc

Rx Resistance Gene

  • pB1-RX.doc

PVX-GFP amplicons

The two amplicon constructs are PUC19-based vectors. These vectors are as described in Cell, 2000 (103), 157-167. PVX-GFP-*CP has a deletion spanning the entire coat protein. PVX-GFP-*TGB-*CP is based on PVX-GFP-*CP in which the entire trible-gene-block encoding the movement proteins (including the p25 suppressor of PTGS) has been removed. Both amplicon constructs are under 35S promoter and Nos terminator. The expression cassettes can be mobilised with a SacI digest and easily subcloned in any binary vector.

  • PVX-GFP-delta CP (Word)
  • PVX-GFP minimal amplicon (Word)

RYMV

  • PJIT60-RYMV.doc

Keywords

Plasmids, Virus vectors, Sequence Data

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Except where otherwised noted, this item's license is described as https://creativecommons.org/licenses/by/4.0/

Relationships

Is supplemented by:
https://doi.org/10.17863/CAM.113581
 https://doi.org/10.17863/CAM.113582
 https://doi.org/10.17863/CAM.113583
 https://doi.org/10.17863/CAM.113580
 https://doi.org/10.17863/CAM.113576
 https://doi.org/10.17863/CAM.113833

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Methods used by the Baulcombe group (Gene expression)