Difference: ProtocolsAcinetobacterBaylyiADP1 (2 vs. 3)

Revision 32022-03-18 - JeffreyBarrick

Line: 1 to 1

META TOPICPARENT	name="ProtocolList"

Acinetobacter baylyi ADP1 Overview

ADP1 Resources

Genome Sequences

Changed:

<
<

- ADP1 Wild-Type (GenBank: NC_005966.1)
  In general, use this genome as a reference when referring to coordinates of genes and features in the ADP1 genome.
  - BLAST a sequence against the ADP1 (WT) genome (at NCBI)
- ADP1 Barrick (GenBank: NC_005966.1)
  Incorporates a small number of mutations found in the WT ADP1 strain that the Barrick lab originally obtained from Valérie de Crécy-Lagard. Use for analyzing NGS sequencing results.
- [[][ADP1-ISx]]
  Strain created in the Barrick lab with all IS1236 elements deleted. (NEEDS LINK)

>
>

- ADP1 type strain (GenBank Format)
  In general, use this genome as a reference when referring to coordinates of genes and features in the ADP1 genome. We added the locations of IS1236 elements to the linked sequence. Otherwise it is the same as the one on NCBI.
  - Original sequence of the ADP1 type strain at NCBI (GenBank: NC_005966.1)
  - BLAST a sequence against this genome at NCBI
- ADP1 Barrick Lab strain (GFF3 Format)
  Incorporates a small number of mutations found in the ADP1 strain that the Barrick lab originally obtained from Valérie de Crécy-Lagard. Use for analyzing NGS sequencing results.
- ADP1-ISx (GFF3 Format)
  Strain created in the Barrick lab with all IS1236 elements deleted.

Other Useful Sequences

Changed:

<
<

- tdk-kanR cassette used for genome editing

>
>

- pBTK622
  Plasmid containing the tdk-kanR cassette used for genome editing.

Functional Genomics
- ADP1 pathways and gene functions (KEGG)

Line: 38 to 39

Plasmids

Changed:

<
<

Common high-copy number E. coli plasmids do not work in ADP1. A synthetic plasmid (pBAV1K) and broad-host-range plasmid (RSF1010) have been used successfully. In our hands, pBAV1K is less reliable. It is also important to note that because plasmid DNA is linearizes when taken up through the competence apparatus, that transformation of plasmids can be significantly less efficient than transformations used to incorporate DNA directly in the chromosome.

>
>

Common high-copy number E. coli plasmids do not work in ADP1.

A synthetic plasmid (pBAV1K) and broad-host-range plasmid (RSF1010) have been used successfully. In our hands, pBAV1K is less reliable. It is also important to note that because plasmid DNA is linearizes when taken up through the competence apparatus, that transformation of plasmids can be significantly less efficient than transformations used to incorporate DNA directly in the chromosome.

Origin	Copy Number	Example
ColE1 (pUC, pBR322, etc.) type plasmids	Do not replicate	NA

View topic | History: r6 < r5 < r4 < r3 | More topic actions...