A Domesticated <i>piggyBac</i> Transposase Plays Key Roles in Heterochromatin Dynamics and DNA Cleavage during Programmed DNA Deletion in <i>Tetrahymena thermophila</i>

Cheng, Chieh-Fang; Vogt, Alexander; Mochizuki, Kazufumi; Yao, Meng-Chao

doi:10.1091/mbc.e09-12-1079

Cited by 147 publications

(251 citation statements)

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“…Previous studies have shown that many heterochromatin components are required for DNA elimination and for the production of viable sexual progeny (Coyne et al, 1999;Mochizuki et al 2002;Malone et al, 2005;Liu et al, 2007;Cheng et al, 2010). DNA elimination in the exconjugants (progeny) of JUB6 MIC-KO was analyzed by using DNA fluorescent in situ hybridization (FISH) with probes complementary to the Tlr1 IESs, which show moderate levels of repetition (Wuitschick et al, 2002).…”

Section: Jub6p Is Important For Dna Eliminationmentioning

confidence: 99%

“…The first group consists of proteins required for the formation of heterochromatin at IESs, including the RNAi machinery components Dcl1p, Twi1p, Giw1p and Ema1p, the histone methyltransferase Ezl1p and the HP1-like protein Pdd1p (Aronica et al, 2008;Coyne et al, 1999;Liu et al, 2004Liu et al, , 2007Malone et al, 2005;Mochizuki and Gorovsky, 2005;Noto et al, 2010). The second group includes proteins that are dispensable for heterochromatin formation but are required for its assembly into heterochromatin bodies: Jub1p, Lia1p, Lia4p, Lia5p, Pdd2p, Tku80p and Tpb2p Rexer and Chalker, 2007;Horrell and Chalker, 2014;Shieh and Chalker, 2013;Liu et al, 2007;Cheng et al, 2010;Lin et al, 2012;Vogt and Mochizuki, 2013;Kataoka and Mochizuki, 2015). Although some of the mechanisms responsible for the former RNAi-directed heterochromatin formation process have been elucidated at the biochemical level, the latter heterochromatin body formation process remains elusive.…”

Section: Introductionmentioning

confidence: 99%

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Heterochromatin aggregation during DNA elimination in Tetrahymena is facilitated by a prion-like protein

Kataoka

Mochizuki

2016

Journal of Cell Science

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Regulated aggregations of prion and prion-like proteins play physiological roles in various biological processes. However, their structural roles in the nucleus are poorly understood. Here, we show that the prion-like protein Jub6p is involved in the regulation of chromatin structure in the ciliated protozoan Tetrahymena thermophila. Jub6p forms sodium dodecyl sulfate (SDS)-resistant aggregates when it is ectopically expressed in vegetative cells and binds to RNA in vitro. Jub6p is a heterochromatin component and is important for the formation of heterochromatin bodies during the process of programmed DNA elimination. We suggest that RNAprotein aggregates formed by Jub6p are an essential architectural component for the assembly of heterochromatin bodies.

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Section: Jub6p Is Important For Dna Eliminationmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Heterochromatin aggregation during DNA elimination in Tetrahymena is facilitated by a prion-like protein

Kataoka

Mochizuki

2016

Journal of Cell Science

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“…These small RNAs are bound by the piwi-related Tetrahymena argonaute proteins Twi1p and Twi11p (Mochizuki et al, 2002;Couvillion et al, 2009;Noto et al, 2015) and are thought to guide heterochromatin targeting through homology recognition, though the targeting mechanism is still unknown. The targeted regions are modified with silencing marks, including specific histone modifications and chromodomain proteins (Taverna et al, 2002;Liu et al, 2004Liu et al, , 2007Yao and Chao, 2005), leading to their excision using a domesticated piggyBac transposase, Tpb2p (Cheng et al, 2010;Chalker and Yao, 2011). Remarkably, injections of dsRNAs into developing cells causes efficient deletion of the corresponding macronuclear DNA from the progeny (Yao et al, 2003).…”

Section: Introductionmentioning

confidence: 99%

Dynamic distributions of long double-stranded RNA in Tetrahymena during nuclear development and genome rearrangements

Woo

Chao

Yao

2016

Journal of Cell Science

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Bi-directional non-coding transcripts and their ∼29-nt small RNA products are known to guide DNA deletion in Tetrahymena, leading to the removal of one-third of the genome from developing somatic nuclei. Using an antibody specific for long double-stranded RNAs (dsRNAs), we determined the dynamic subcellular distributions of these RNAs. Conjugation-specific dsRNAs were found and show sequential appearances in parental germline, parental somatic nuclei and finally in new somatic nuclei of progeny. The dsRNAs in germline nuclei and new somatic nuclei are likely transcribed from the sequences destined for deletion; however, the dsRNAs in parental somatic nuclei are unexpected, and PCR analyses suggested that they were transcribed in this nucleus. Deficiency in the RNA interference (RNAi) pathway led to abnormal aggregations of dsRNA in both the parental and new somatic nuclei, whereas accumulation of dsRNAs in the germline nuclei was only seen in the Dicer-like gene mutant. In addition, RNAi mutants displayed an early loss of dsRNAs from developing somatic nuclei. Thus, long dsRNAs are made in multiple nuclear compartments and some are linked to small RNA production whereas others might participate in their regulations.

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“…The clones 6-1, 9-2, 9-6, 17-1 of TTHERM_00301940 KO cells were selected for further study. TTHERM_00301940 is exclusively expressed during conjugation and many conjugation-specific genes are required for DNA elimination (Mochizuki et al 2002;Taverna et al 2002;Liu et al 2007;Cheng et al 2010;Shieh and Chalker 2013;Woehrer et al 2015); we sought to determine whether TTHERM_00301940 is also involved in DNA elimination. TTHERM_00301940 KO strains (6-1 3 9-6 [= cross 1 in Table 1] or 9-2 3 17-1 [= cross 2 in Table 1]) were mated, and the DNA elimination in their exconjugants (progeny) was analyzed by DNA FISH using probes complementary to the Tlr1 element.…”

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confidence: 99%

“…In contrast to the gene KO strategies, RNAi KD can be done in a shorter period of time and is thus suitable for high-throughput genetic screening. However, RNAi KD often only incompletely shuts down expression of a target gene (Howard-Till and Yao 2006;Cheng et al 2010;Chung and Yao 2012;Lukaszewicz et al 2013) and may thus result in the misinterpretation of the gene function. During the development of the new MAC of Tetrahymena, .8000 DNA segments called internal eliminated sequences (IESs) were reproducibly eliminated.…”

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Targeted Gene Disruption by Ectopic Induction of DNA Elimination in Tetrahymena

Hayashi¹,

Mochizuki

2015

Genetics

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Tetrahymena is a useful eukaryotic model for biochemistry and molecular cell biology studies. We previously demonstrated that targeted ectopic DNA elimination, also called co-Deletion (coDel), can be induced by the introduction of an internal eliminated sequence (IES)-target DNA chimeric construct. In this study, we demonstrate that coDel occurs at most of the loci tested and can be used for the production of somatic gene KO strains. We also showed that coDel at two loci can be simultaneously induced by a single transformation; thus, coDel can be used to disrupt multiple gene loci in a single cell. Therefore, coDel is a useful tool for functional genetics in Tetrahymena and further extends the usefulness of this model organism.KEYWORDS Tetrahymena; DNA elimination; RNAi; gene knockout T HE ciliated protozoan Tetrahymena thermophila can grow at an exceptionally high rate (its doubling time is approximately 2 hr) and can reach a high density (a few million cells per milliliter) under simple and inexpensive culture conditions (reviewed in Orias et al. 2000). In combination with robust genetic manipulation methods (reviewed in Chalker 2012), Tetrahymena is a useful model eukaryote for biochemistry and molecular cell biology studies (reviewed in Collins and Gorovsky 2005).Three strategies for loss-of-function genetic studies have been established for this organism. The first strategy is a germline knockout (KO), in which one of the two gene copies in the diploid micronucleus (MIC) is replaced with a drug-resistance gene by homologous recombination, and two heterozygous strains are then sexually crossed to obtain a homozygous germline KO strain (Cassidy-Hanley et al. 1997). The second strategy is somatic KO, in which one of the 45 copies of a gene in the polyploid macronucleus (MAC) is replaced with a drugresistance gene by homologous recombination, and "phenotypic assortment" is used to obtain cells with the drug-resistance gene at all loci (Merriam and Bruns 1988). Phenotypic assortment is possible because MAC chromosomes are randomly segregated into daughter cells in vegetative cell division and a stepwise increase of the drug in culture selects for cells that have more drug-resistance genes. The final strategy is gene knockdown (KD) by RNA interference (RNAi), in which a construct expressing long hairpin RNA that is complementary to the gene of interest is introduced into a nonessential locus in the MAC and small RNAs produced from the hairpin RNA posttranscriptionally silence the expression of the gene (HowardTill and Yao 2006).Although the first two gene KO strategies have been reliably used to study individual gene functions, they are not suitable for high-throughput genetic screening because the integration of a KO construct into the MIC germline occurs at very low efficiency and the phenotypic assortment process used in somatic KOs require the careful control of drug concentrations in each strain and culture step. Moreover, it takes 1 month to obtain KO strains using these methods. For germline KO, t...

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A Domesticated piggyBac Transposase Plays Key Roles in Heterochromatin Dynamics and DNA Cleavage during Programmed DNA Deletion in Tetrahymena thermophila

Cited by 147 publications

References 45 publications

Heterochromatin aggregation during DNA elimination in Tetrahymena is facilitated by a prion-like protein

Heterochromatin aggregation during DNA elimination in Tetrahymena is facilitated by a prion-like protein

Dynamic distributions of long double-stranded RNA in Tetrahymena during nuclear development and genome rearrangements

Targeted Gene Disruption by Ectopic Induction of DNA Elimination in Tetrahymena

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