Difference between revisions of "Part:BBa K2889000:Design"

Revision as of 05:19, 8 October 2018

pSB1C3-IL7-AS-S2

Assembly Compatibility:

10
COMPATIBLE WITH RFC[10]
12
COMPATIBLE WITH RFC[12]
21
INCOMPATIBLE WITH RFC[21]
Illegal BglII site found at 198
23
COMPATIBLE WITH RFC[23]
25
COMPATIBLE WITH RFC[25]
1000
COMPATIBLE WITH RFC[1000]

Design Notes

We wanted to investigate which domain is essential for the function of IL7-AS. We cloned the truncated sequences of IL7-AS (IL7-AS-S2) into pSB1C3 for submitting to IGEM 2018 and inserted IL7-AS-S2 into pCDNA3.1 to study the function.

Source

We cloned the truncated sequences of IL7-AS (IL7-AS-S2,411 bp) from human cells. 1.1 Amplification of IL7-AS-S2 fragments from human cell line. First we amplified IL7-AS-S2 using primers. After that, we purified the PCR products by PCR Purification Kit and digested them with restriction enzymes EcoRI and PstI (Fig 1). 1.2 Digested PSB1C3 vector. We digested the PSB1C3 vectors with EcoRI and PstI (Fig 2). https://parts.igem.org/File:Digested_the_PSB1C3_vectors_with_EcoRI_and_PstI.jpeg 1.3 Ligation of purified IL7-AS-S2 fragments to pSB1C3 vector. IL7-AS-S2 fragments were ligated to PSB1C3 vector. Then we selected the positive clones by PCR and sequencing (Fig 3).

References

Roux, B. T., Heward, J. A., Donnelly, L. E., Jones, S. W., and Lindsay, M. A. (2017) Catalog of Differentially Expressed Long Non-Coding RNA following Activation of Human and Mouse Innate Immune Response. Frontiers in immunology 8, 1038

@@ Line 16: / Line 16: @@
 .1 Amplification of IL7-AS-S2 fragments from human cell line.
 First we amplified IL7-AS-S2 using primers. After that, we purified the PCR products by PCR Purification Kit and digested them with restriction enzymes EcoRI and PstI (Fig 1).
-https://parts.igem.org/File:Amplification_of_IL7-AS_and_IL7-AS-S2.jpeg
+https://static.igem.org/mediawiki/parts/e/e0/Amplification_of_IL7-AS_and_IL7-AS-S2.jpeg
 .2	Digested PSB1C3 vector.
 We digested the PSB1C3 vectors with  EcoRI and PstI (Fig 2).