Team:Hawaii/Construction of Broad-Host-Range Expression Vector

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Latest revision as of 01:10, 16 August 2008

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Construction of Broad-Host-Range Expression Vector from pRL1383a and Other Parts

This expression vector will pull parts from the RSF1010 derived broad-host-range plasmid pRL1383a, the self-transmissible plasmid RP4 and also from available BioBrick parts. These parts will be obtained through either PCR amplification from the original DNA, by synthetically constructing them as outlined in Silver's method for overlapping oligonucleotides, and finally through extraction from the BioBrick parts registry.

The obtained parts will then be maintained on seperate plasmids then later compiled onto the BioBrick Base Vector, [http://partsregistry.org/Part:BBa_I51020 BBa_I51020]. The mobility of this vector will be tested by first transforming into E. coli then conjugatively transferred to SynechocystisPCC6803, followed by the final test of cloning in genes and testing their expression in both E. coli and SynechocystisPCC6803.

Design

Methods

Design Primers
Design overlapping oligonucleotides and oligonucleotide inserts
Selection of additional BioBrick parts
Lay-out of the new vector

Results

These genes were amplified from pRL1383a in all cases except for the P1 lytic region which will be amplified from a BioBrick plasmid: pSB2K3.

pRL1383a Genes w/ BioBrick Ends

name	primer	Tm	Reviewed By	Notes
aadA_fp._sb.1	cctTTCTAGatgagggaagcggtgatcg	59.4/65.7 C	NW	isolates aadA from ATG to TAA-TAA
aadA_rp._sb.1	aaggCTGCAGCGGCCGCTACTAGTAttattatttgccgactaccttgg	55.4/74.5	NW	isolates aadA from ATG to TAA-TAA
OmegaInterposon_fo._sb.1	cctTTCTAGAGggtgattgattgagcaagc	54.5/65	NW	mixture of 4 products, 2/4 correct
OmegaInterposon_ro._sb.1	aaggCTGCAGCGGCCGCTACTAGTAggtgattgattgagcaagc	54.5/75.5	NW	mixture of 4 products, 2/4 correct
pRL1383aOriV_fb._sb.1	cctTTCTAGAGgaacccctgcaataactgtc	56.3/65.9	NW
pRL1383aOriV_rb._sb.1	aaggCTGCAGCGGCCGCTACTAGTAgctgaatgatcgaccgagac	58/76.2	NW
pRL1383aRep_fp._sp.1	cctTTCTAGatgaagaacgacaggactttgc	58.9/64.9	NW	Begins with RepB
pRL1383aRep_rb._sb.1	aaggCTGCAGCGGCCGCTACTAGTAcctatggagctgtgcggca	62.2/78.5	NW	Ends RepC terminator.8/2:the terminator is missing the last C.
p1lytic_fb._sb.1	atGAATTCGCGGCCGCTTCTAGAGcgcagttgcaaaccctcac	59.5/76.2	NW	E-N-X(front ligation);inducible high-copy-#, incl. P_lac;from pSB2K3
p1lytic_rp._sb.1	cTACTAGTATTAttaccctctgaatcctgccg	59.2/63.5	NW	S(front ligation), ends w/(TAATAA);induced high-copy-#;from pSB2K3

The origin of conjugative transfer will be synthetically constructed using the Overlapping Oligonucleotides method from the Silver Lab [1].

RP4 Origin of Transfer Sequences for Oligonucleotide Extension

name	oligonucleotide set	Reviewed by	Notes
oriT1_ob._na.1	ctagaggaataagggacagtgaagaaggaacacccgctcg	NW	complement oriT4
oriT2_ob._na.1	cgggtgggcctacttcacctatcctgcccggctgacgccg	NW	complement of oriT5
oriT3_ob._na.1	ttggatacaccaaggaaagtctacatactagtagcggccgctgca	NW	complement of oriT6
oriT4_ob._na.1	GCGGCCGCTACTAGTAtgtagactttccttggtg	NW
oriT5_ob._na.1	tatccaacggcgtcagccgggcaggataggtgaagtaggcc	NW
oriT6_ob._na.1	cacccgcgagcgggtgttccttcttcactgtcccttattcCT	NW

BioBricks Extracted from Registry

name	Function	Combined with?
[http://partsregistry.org/Part:pSB1A7 pSB1A7]	high copy BioBrick vector, Amp^R, insulated	Storage for oriV, oriT
[http://partsregistry.org/Part:BBa_I51020 BBa_I51020]	BioBrick Base Vector	final assembly of all parts
[http://partsregistry.org/Part:BBa_I14032 BBa_I14032]	lac promoter	rep region, aadA region
[http://partsregistry.org/Part:BBa_B0034 BBa_B0034]	RBS PoPS=1.0	rep region, aadA region
[http://partsregistry.org/Part:BBa_B0015 BBa_B0015]	Double terminator	aadA region, P1 lytic region
[http://partsregistry.org/Part:BBa_J23012 BBa_J23012]	aadA BioBrick	combine with lac promoter and double terminator

Discussion

Make Parts

I am making the parts several different ways: 1. PCR amplification, 2. synthetic construction of overlapping oligonucleotides, 3. extraction from BioBrick Registry.

PCR Amplification of pRL1383a

Each of these experiments can be found at the link above. This will include amplification products from other plasmids besides pRL1383a.

Oligonucleotide Assemby

The experiment and results can be found on the link above under the heading: "2 Construction of OriT from RP4 using Overlapping Oligonucleotides: Attempt 1"

Extraction of BioBrick Parts from Registry

Some parts were extracted from BioBrick registry, the experiments and results will be included in the link above.

Ligation of Parts

Experiments and results found in link above.

References

http://openwetware.org/wiki/Silver:_Oligonucleotide_Inserts Silver Lab, Overlapping Oligonucleotides Inserts Protocol.

[http://manoa.hawaii.edu/ ][http://manoa.hawaii.edu/ovcrge/ ][http://www.ctahr.hawaii.edu ]

@@ Line 12: / Line 12: @@
 * Design Primers
-* Design overlapping oligonucleotides
+* Design overlapping oligonucleotides and oligonucleotide inserts
 * Selection of additional BioBrick parts
 * Lay-out of the new vector
@@ Line 18: / Line 18: @@
 === Results ===
-* These genes will be PCR amplified from pRL1383a in all cases except for the P1 lytic region which will be amplified from a BioBrick plasmid: pSB2K3.
+* These genes were amplified from pRL1383a in all cases except for the P1 lytic region which will be amplified from a BioBrick plasmid: pSB2K3.
 '''pRL1383a Genes w/ BioBrick Ends'''
@@ Line 177: / Line 177: @@
 :*Some parts were extracted from BioBrick registry, the experiments and results will be included in the link above.
+==[[Team:Hawaii/Ligation of pRL1383a Parts|Ligation of Parts]]==
+:* Experiments and results found in link above.
 == References ==