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June 1^st 2012

Vector mini-prep: Moth_gene carrying pTrcHis2A transformed into TOP10 strain

We extracted the vector carrying Moth_1201, 1202, 1204, 2314, 1197, 1198, 1199, 0109, 1191, 1516 from transformed E. coli TOP10 strain.

Results

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PCR for TOPO cloning

With the extracted vectors, we performed PCR to amplify each inserted genes to further use them for TOPO vector cloning. As we always do, elongation time was set as 1 min/kb.

Results

With these amplified genes, we performed PCR purification. Concentration and purity are as follows.

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June 2^nd 2012

PCR amplification of control gene

We PCR amplified a gene to use as a negative control when evaluating the expression result of TOPO cloning.

Results

Control gene is about 800nt long. We purified this gene and its concentration was 216.0 ng/µl with purity of 1.80.

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TOPO cloning

With the PCR amplified and purified genes, we performed TOPO cloning by inserting those genes into pBAD TOPO vector to examine the expression of genes with different inducing agent. Ligated TOPO vector was transformed into E. coli TOP10 strain by heat shock transformation method. Transformed cells were spread on LB agar plate for further colony check.

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Moth_0109, 1191, 1516 expression check

Cells transformed with pTrcHis2A vectors carrying each of the genes Moth_0109, 1191, 1516 were seeded to examine the expression of each gene. As this vector carries lac operon, genes are induced by treating IPTG of proper amount. Six hours after induction, cell culture will be harvested and the amount of target proteins will be assessed by SDS PAGE. (Both soluble and insoluble fractions of proteins were assessed.)

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June 3^rd 2012

Colony PCR: 12 transformed genes and control gene

We performed colony PCR with 12 transformed samples and a control to verify if the transformation of cloned TOPO vector into TOP10 strain was successful. Total three colonies were selected from each samples.

Results

Some bands of samples failed to appear in the right place such as Moth_0109 and 2314.

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Re-colony PCR: Moth_0109, 2314

Since two samples did not show any successful result in colony PCR and we just gave it another try.

Results

As we can see, Moth_0109 genes amplified through colony PCR has different length compared to the gene construct originally inserted into the vector. This means that Moth_0109 failed to be cloned into the vector and thus transformation was not successful either.

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Moth_0109, 1191, 1516 SDS PAGE

With the seeded samples on 6/2, we induced the cell cultures and performed SDS PAGE to see the expression of each gene.

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Colony selection and seeding for sequencing

From successfully transformed samples, we selected colonies and cultured them for sequencing. Once their vectors are extracted, they will be sent to Xenotech for sequencing.

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June 4^th 2012

Colony PCR: Moth_0109 (10 samples)

Since Moth_0109 gene did not show any satisfactory result from colony PCR, we tried it again to figure out the problem.

Results

PCR results showed multiple bands again. Moreover, bands are not in the correct position.

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Vector mini-prep for sequencing

We extracted vectors from 11 successfully transformed samples of TOP10.

Results

Among these samples, those whose concentration exceeded 100 ng/µl were sent for sequencing.

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June 5^th 2012

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June 6^th 2012

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June 7^th 2012

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June 8^th 2012

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June 9^th 2012

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June 10^th 2012

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June 11^th 2012

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June 12^th 2012

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June 13^th 2012

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June 14^th 2012

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June 15^th 2012

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June 16^th 2012

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June 17^th 2012

June 18^th 2012

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June 19^th 2012

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June 20^th 2012

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June 21^st 2012

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June 22^nd 2012

Moth_0109, 1202 colony PCR

Results

There is no band in the gel. We failed TOPO cloning of Moth 0109, 1202.

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June 23^rd 2012

Moth_0109, 1202 colony PCR

Results

There is no band in the gel. We failed TOPO cloning of Moth 0109, 1202.

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June 24^th 2012

Moth_0109, 1202 PCR result

Results

We failed Moth_0109, 1202 TOPO cloning so we tried it again. The PCR band is correct. It means we were successful to make insert DNA.

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pBAD TOPO enzyme cut extraction

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Results

We didn’t have the TOPO solution anymore. So we tried to reuse the TOPO vector from the other cloned vector. We cut the vector using same restriction enzyme with Moth 0109, 1202 insert and extracted the vector.

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June 25^th 2012

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June 26^th 2012

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June 27^th 2012

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June 28^th 2012

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June 29^th 2012

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June 30^th 2012

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