piggyBac转座酶的瞬时表达对莱茵衣藻体内piggyBac转座子的作用

Abstract
Figure/Table
References
Related Citation (2)

Download: PDF (6331 KB) HTML (1 KB)
Export: BibTeX | EndNote (RIS)

Abstract The cut-and-paste piggyBac (PB) transposon system has been shown to be a useful tool for genetic modification in a number of organisms including mammals, insects, and yeast. However, little is known whether it is active in the green microalga Chlamydomonas reinhardtii. In this study, we constructed stable PB element-containing C. reinhardtii strains bearing either a single copy or multiple copies of PB element. Subsequently, we transiently expressed TPase or codon-optimized crTPase in the PB element-containing strains to assay for transposition of PB element using restriction fragment length polymorphism (RFLP) methodology. Our analyses show that initial RFLP patterns of PB element are altered in cells one week and two weeks after plasimds containing TPase or crTPase expression cassette. The size of PB element-containing fragment remained unchanged in TR1 cells after transformation of the pJR38 plasmid containing no TPase or crTPase sequences. This result indicated that PB element was stable without TRpase or crTPase activity in cells. On the contrary, RFLP patterns of the PB element were altered 1 week and 2 weeks after transient expression of TPase or crTPase in TR1 or TR3 cells. For example, a fragment of 1.5 kb containing PB element was present in TR1 prior to transformation of TPase-containing plasmid. One week after transformation, one initial fragment of 1.5 kb and 3 new fragments of 2.8, 4.2 and 6.5 kb disappeared and appeared, respectively, suggesting transposition of the PB element occurred in TR1 cells. Two weeks after transformation, the size of all 3 fragments changed again, implying that transposition persists. In TR3, 1 week after the transformation, 3 fragments of 1.5, 3 and 4 kb and 1 fragment of 6.5 kb remained unchanged and disappeared, respectively. Meanwhile, a new fragment of 2.8 kb appeared. The RFLP pattern was hardly altered again 2 week after the transformation. These results indicated that the sizes of PB element-containing fragments changed, implying the PB element transposed after introducing the TPase and crTPase activities in C. reinhardtii TR1 and TR3 strains. Furthermore, to test whether PB element had been transposed in these cells, we examined the presence of a new joint generated by excision of the PB element in the genome. To this end, primers flanking to the new joint were applied for PCR analysis using the genomic DNA derived from the colonies. Clearly, excision event of the PB element was detected. This result supports the results that PB transposon system is active in C. reinhardtii. To find out the reason that the cells could survive the transposition of PB element, PCR fragments containing the PB element excision joint were subjected to nucleotide sequence analysis. Alignment of the sequences indicated that cells from the colonies suffered from illegitimate excision of PB element. The study shows that illegitimate excision of PB element occasionally occurs at the short repeat sequences 5'-TTT-3' and 5'-ACGCAG-3', but the standard excision site 5'-TTAA-3'. This study shows that the TPase and crTPase are active in transposition of PB element in C. reinhardtii. Hence, we propose that PB transposon systems can be adopted for genome modification in C. reinhardtii.

Key words： Genetic modification Green microalgae Illegitimate excision PiggyBac transposon RFLP

Received: 22 June 2016 Published: 01 October 2016

	Service

	E-mail this article
	Add to my bookshelf
	Add to citation manager
	E-mail Alert
	RSS
	Articles by authors
	ZI Shu-Yuan


	HE Jing
	YANG Xiao-Kang
	LIU Jian-Hua

Cite this article:

ZI Shu-Yuan,HE Jing,YANG Xiao-Kang, et al. Transposition of PiggyBac (PB) Element is Attributed to Transient Expression of PB Transposase in Chlamydomonas reinhardtii [J]. , 2016, 24(11): 1643-1651.

URL:

http://journal05.magtech.org.cn/Jwk_ny/EN/ OR http://journal05.magtech.org.cn/Jwk_ny/EN/Y2016/V24/I11/1643

Chen YT, Furushima K, Hou PS, Ku AT, Deng JM, Jang CW, et al. 2010. PiggyBac
transposon-mediated, reversible gene transfer in human embryonic stem cells. Stem Cells
Dev. 19: 763-771.
Davies JP, Yildiz FH, Grossman AR. 1999. Sac3, an Snf1-like serine/threonine kinase that positively and negatively regulates the responses of Chlamydomonas to sulfur limitation.
Plant Cell. 11: 1179-1190.
Ding S, Wu X, Li G, Han M, Zhuang Y, Xu T. 2005. Efficient transposition of the piggyBac
(PB) transposon in mammalian cells and mice. Cell. 122: 473-483.
Fischer JA, Giniger E, Maniatis T, Ptashne M. 1988. GAL4 activates transcription in Drosophila. Nature. 332: 853-856.
Fraser MJ, Ciszczon T, Elick T, Bauser C. 1996. Precise excision of TTAA-specific
lepidopteran transposons piggyBac (IFP2) and tagalong (TFP3) from the baculovirus genome
in cell lines from two species of Lepidoptera. Insect Mol Biol. 5: 141-151.
Gonzalez-Ballester D, Pootakham W, Mus F, Yang W, Catalanotti C, Magneschi L, et al.
2011. Reverse genetics in Chlamydomonas: a platform for isolating insertional mutants. Plant Methods. 7: 24.
Gorman DS, Levine RP. 1965. Cytochrome f and plastocyanin: their sequence in the
photosynthetic electron transport chain of Chlamydomonas reinhardi. Proc Natl Acad Sci U S
A. 54: 1665-1669.
Harris EH. 1998. The Chlamydomonas Sourcebook. Academic Press, San Diego, CA, USA.
Heitzer M, Eckert A, Fuhrmann M, Griesbeck C. 2007. Influence of codon bias on the
expression of foreign genes in microalgae. Transgenic Microalgae as Green Cell Factories.
616: 46-53.
Ibrahim F, Rohr J, Jeong WJ, Hesson J, Cerutti H. 2006. Untemplated oligoadenylation
promotes degradation of RISC-cleaved transcripts. Science. 314: 1893.
Jiang W, Brueggeman AJ, Horken KM, Plucinak TM, Weeks DP. 2014. Successful transient
expression of Cas9 and single guide RNA genes in Chlamydomonas reinhardtii. Eukaryot
Cell. 13: 1465-1469.
Kim H, Kim K, Kim J, Kim SH, Yim J. 2012. Mutagenesis by imprecise excision of the
piggyBac transposon in Drosophila melanogaster. Biochem Biophys Res Commun. 417: 335-
339.
Lobo NF, Fraser TS, Adams JA, Fraser MJ, Jr. 2006. Interplasmid transposition demonstrates
piggyBac mobility in vertebrate species. Genetica. 128: 347-357.
Lumbreras V, Stevens DR, Purton S. 1998. Efficient foreign gene expression in
Chlamydomonas reinhardtii mediated by an endogenous intron. Plant Journal. 14: 441-447.
Merchant SS, Prochnik SE, Vallon O, Harris EH, Karpowicz SJ, Witman GB, et al. 2007.
The Chlamydomonas genome reveals the evolution of key animal and plant functions.
Science. 318: 245-250.
Neupert J, Karcher D, Bock R. 2009. Generation of Chlamydomonas strains that efficiently
express nuclear transgenes. Plant Journal. 57: 1140-1150.
Ohresser M, Matagne RF, Loppes R. 1997. Expression of the arylsulphatase reporter gene
under the control of the nit1 promoter in Chlamydomonas reinhardtii. Curr Genet. 31: 264-
271.
Rasala BA, Lee PA, Shen Z, Briggs SP, Mendez M, Mayfield SP. 2012. Robust expression
and secretion of Xylanase1 in Chlamydomonas reinhardtii by fusion to a selection gene and
processing with the FMDV 2A peptide. PLoS One. 7: e43349.
Shimogawara K, Fujiwara S, Grossman A, Usuda H. 1998. High-efficiency transformation of
Chlamydomonas reinhardtii by electroporation. Genetics. 148: 1821-1828.
Stevens DR, Rochaix JD, Purton S. 1996. The bacterial phleomycin resistance gene ble as a
dominant selectable marker in Chlamydomonas. Mol Gen Genet. 251: 23-30.
Tam LW, Lefebvre PA. 1993. Cloning of flagellar genes in Chlamydomonas reinhardtii by
DNA insertional mutagenesis. Genetics. 135: 375-384.
Tam LW, Lefebvre PA. 1995. Insertional mutagenesis and isolation of tagged genes in
Chlamydomonas. Methods Cell Biol. 47: 519-523.
Wilson MH, Coates CJ, George AL, Jr. 2007. PiggyBac transposon-mediated gene transfer in
human cells. Mol Ther. 15: 139-145.
Zhao T, Li G, Mi S, Li S, Hannon GJ, Wang XJ, Qi Y. 2007. A complex system of small
RNAs in the unicellular green alga Chlamydomonas reinhardtii. Genes Dev. 21: 1190-1203.