The Nucleus v0.1.0 distribution plate is the first release of the physical DNA encoding Nucleus content components and modules, available under the OpenMTA.
Table of Contents
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<img src="/icons/key_gray.svg" alt="/icons/key_gray.svg" width="40px" /> Key Information
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| Backbone |
pOpen v3 |
| Antibiotic Resistance |
Amp |
| Concentration (fmol) |
10 |
| Total volume (ul) |
10 |
| Sequence Information |
[Github] |
Plate Map
|
1 |
2 |
3 |
4 |
5 |
6 |
7 |
8 |
9 |
10 |
11 |
12 |
Category |
| A |
AlaRS |
ArgRS |
AsnRS |
AspRS |
CysRS |
GlnRS |
GluRS |
GlyQS-DualHis |
HisRS |
IleRS |
LeuRS |
LysRS |
PURE |
| B |
MetRS |
PheST-DualHis |
ProRS |
SerRS |
ThrRS |
TrpRS |
TyrRS |
ValRS |
MTF |
IF1 |
IF2 |
IF3 |
PURE |
| C |
EF-G |
EF-Tu |
EF-Ts |
RF1 |
RF2 |
RF3 |
RRF |
AK-Gg |
CK-Gg |
NDK |
PPiase |
T7RNAP |
PURE |
| D |
GlyS |
GlyQ |
GlySQ |
GlyQS |
PheS |
PheT |
PheST |
PheTS |
AK-Sc-1 |
AK-Sc-2 |
AK-Oc |
AK-Ec |
PURE |
| E |
CK-Oc |
plamGFP-Chimeric |
plamGFP-PURE |
plamGFP-TXTL |
mmilCFP |
meleRFP |
cjBlue |
cjBlue-lacO |
cjBlue-lacO-His6 |
eforRed |
eforRed-lacO |
eforRed-lacO-His6 |
PURE / Rep |
| F |
PURET7-1 |
PURET7-2 |
PURET7-3 |
PURET7-4 |
PURET7-5 |
PURET7-6 |
PURET7-7 |
PURET7-8 |
PURET7-9 |
PURET7-10 |
amajLime |
gfasPurple |
T7 / Rep |
| G |
tetR |
lacI |
pT7-tetO |
pT7-lacO |
pT7-tetO-lacO |
pT7-lacO-tetO |
|
|
|
|
|
|
Module |
| H |
UTR1 |
RBS |
tT7 |
tT7hyb6 |
tT7hyb10 |
pOpenv3-MCL0 |
|
|
|
|
|
|
MoClo |
Contents
The content of the plate is described in the DNA Distribution document. In general, the plate is arrayed by plasmid category:
- PURE genes occupy the first three rows (A-C), in the gene ordering originally published by Shimizu, et al (2001).
- Row D contains alternative versions of the PURE genes, such as different designs for the two-subunit tRNA synthetases, and metabolic enzymes sourced from different organisms as have been used in the literature.
- Row E contains open measurement reporters.
- Row F contains T7 promoter variants engineered to span two orders of magnitude of expression, for direct testing or use as a MoClo level 0 promoter part.
- Row G contains inducible modules for use in the PURE cell free system.
- Row H contains several basic MoClo level 0 parts for assembly of level 1 transcription units.
Technical Information
- All DNA is encoded on the high-copy pOpen v3 plasmid, in the Nucleus DNA architecture.
- All plasmids on the plate are Ampicillin / Carbenicillin resistant.
- Each construct is normalized to 10 fmol / uL and provided as 10 uL total.
- Plates are sealed with slit silicon plate seals and lids. DNA can be extracted through the slits in the seal without removing it.
- Multichannel pipetting through the slit seal is very difficult.
- Exercise caution if removing the seal—be very gentle, or the vacuum produced will pull sample from the well and potentially cross-contaminate the wells.
- DNA may have shifted in transit—spin down the plate before using it in downstream work.
Getting Started
We recommend sub-cloning the DNA into an appropriate cloning strain such as DH5-alpha or NEB Stable, and preparing more high concentration DNA for downstream use.
- Spin down the plate in a tabletop plate spinner, or a centrifuge at 2000g for 1 minute.