Revision as of 02:03, 2 November 2017

tRNAPhe-MS2

tRNA^Phe-MS2 co-purification construct. Contains a T7 promoter -10 followed by tRNA Phe, two MS2 RNA aptamers and a double terminator. To be used in conjunction with BBa_K2109108.

tRNA Purification

Both BBa K2443038 and BBa_K2109108 were overexpressed individually in E. coli BL21-Gold (DE3) cells. Upon which time the cells were lysed, the lysate combined, and applied to a Nickel Sepharose affinity column. In order to cleave the RNA, 1 µM of DNA oligo was added to the column, as well as varying amounts of RNase H. Incubation times on the column with RNase H and DNA oligo varied from 2 hours (Figure 3) to 12 hours (Figure 4), and the amount of RNase H used varied from 10 units to 100 units (Figure 3 and 4). Based upon the varied conditions, a longer incubation time had the greatest effect on tRNA cleavage efficiency with units of RNase H being optimal between the range of 5-50. With these improvements from our initial attempt at tRNA cleavage we successfully purified tRNA^Phe, as shown in Figure 4.

For more information on the design, see the "http://2017.igem.org/Team:Lethbridge/Design#anchor5" tRNA purification section

Figure 3 - Preliminary tRNA^Phe Purification. 12% 8M urea PAGE run for 45 mins at 300 V. All concentrated fractions were phenol chloroform extracted, ethanol precipitated and re-suspended in 30 µL of ddH₂O. Lanes are as follows: 1- tRNA fraction with 20 units of RNase H added; 2- concentrated tRNA fraction 20 units of RNase H added; 3- concentrated MS2 fraction 1 20 units of RNase H added; 4- concentrated MS2 fraction 2 20 units of RNase H added; 5- tRNA standard (76 nt).

Figure 4 - Successful tRNA^Phe Purification. 12% 8M urea PAGE run for 45 mins at 300 V. All fractions were phenol chloroform extracted, ethanol precipitated and re-suspended in 30 µL of ddH₂O. Lanes are as follows - 1- MS2 fraction 25 units of RNase H added; 2- tRNA fraction 25 units of RNase H added; 3- MS2 fraction 50 units of RNase H added; 4- tRNA fraction 50 units of RNase H added; 5- MS2 fraction 100 units of RNase H added; 6- tRNA fraction 100 units of RNase H added; 7- MS2 fraction 10 units of RNase H added; 8- tRNA elution 10 units of RNase H added; 9- tRNA standard (76 nt).

Sequence and Features

Assembly Compatibility:

10
COMPATIBLE WITH RFC[10]
12
COMPATIBLE WITH RFC[12]
21
COMPATIBLE WITH RFC[21]
23
COMPATIBLE WITH RFC[23]
25
COMPATIBLE WITH RFC[25]
1000
COMPATIBLE WITH RFC[1000]

@@ Line 11: / Line 11: @@
 <p>Both BBa K2443038 and BBa_K2109108 were overexpressed individually in <i>E. coli</i> BL21-Gold (DE3) cells. Upon which time the cells were lysed, the lysate combined, and applied to a Nickel Sepharose affinity column. In order to cleave the RNA, 1 µM of DNA oligo was added to the column, as well as varying amounts of RNase H. Incubation times on the column with RNase H and DNA oligo varied from 2 hours (Figure 3) to 12 hours (Figure 4), and the amount of RNase H used varied from 10 units to 100 units (Figure 3 and 4). Based upon the varied conditions, a longer incubation time had the greatest effect on tRNA cleavage efficiency with units of RNase H being optimal between the range of 5-50. With these improvements from our initial attempt at tRNA cleavage we successfully purified tRNA<sup>Phe</sup>, as shown in Figure 4.</p>
-<p>  For more information on the design,  see the "http://2017.igem.org/Team:Lethbridge/Design#anchor5" tRNA purification</a> section here.</p>
+<p>  For more information on the design, see the "http://2017.igem.org/Team:Lethbridge/Design#anchor5" tRNA purification section</p>
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Difference between revisions of "Part:BBa K2443038"

Revision as of 02:03, 2 November 2017

tRNA Purification