Tandem inverted repeat system for selection of effective transgenic RNAi strains in <i>Chlamydomonas</i>

Rohr, Jennifer; Sarkar, Nandita; Balenger, Susan L.; Jeong, Byeong‐ryool; Cerutti, Heriberto

doi:10.1111/j.1365-313x.2004.02227.x

Cited by 150 publications

(212 citation statements)

References 73 publications

(222 reference statements)

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“…Archaeplastida Chlamydomonas reinhardtii Rohr et al (2004) and Schroda (2006) Arabidopsis thaliana Llave et al (2002) and and Watson et al (2005) Direct b Matzke and Birchler (2005) and Zilberman et al (2003) Chan et al (2004) and Matzke and Birchler (2005) Chen ( Aspergillus nidulans Hammond and Keller (2005) among the RNAi-positive organisms listed in Table 1 is Giardia intestinalis that encodes a protein with a well-defined PIWI domain fused to a highly divergent PAZ domain. However, Giardia protein-encoding genes are notoriously fast-evolving compared with those of most other eukaryotes (Richards and Cavalier-Smith 2005), which might explain the poor conservation of the PAZ domain.…”

Section: Phytophthora Infestansmentioning

confidence: 99%

“…RdRPs are not as widely distributed among eukaryotes as Ago-Piwi and Dicer-like proteins (Table 1). Even though RNAi occurs in animals (Schwarz et al 2002;Stein et al 2003), Chlamydomonas reinhardtii (a green alga) (Rohr et al 2004;Schroda 2006), and T. brucei ), RdRPs were not detected in their genomes (Table 1), with the exception of C. elegans and Branchiostoma floridae (AAQ10792). In Aspergillus nidulans it has been experimentally demonstrated that RNAi induced by an inverted repeat transgene does not require any of the two RdRPs encoded in the genome (Hammond and Keller 2005).…”

Section: Phytophthora Infestansmentioning

confidence: 99%

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On the origin and functions of RNA-mediated silencing: from protists to man

2006

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Double-stranded RNA has been shown to induce gene silencing in diverse eukaryotes and by a variety of pathways. We have examined the taxonomic distribution and the phylogenetic relationship of key components of the RNA interference (RNAi) machinery in members of five eukaryotic supergroups. On the basis of the parsimony principle, our analyses suggest that a relatively complex RNAi machinery was already present in the last common ancestor of eukaryotes and consisted, at a minimum, of one Argonautelike polypeptide, one Piwi-like protein, one Dicer, and one RNAdependent RNA polymerase. As proposed before, the ancestral (but non-essential) role of these components may have been in defense responses against genomic parasites such as transposable elements and viruses. From a mechanistic perspective, the RNAi machinery in the eukaryotic ancestor may have been capable of both small-RNA-guided transcript degradation as well as transcriptional repression, most likely through histone modifications. Both roles appear to be widespread among living eukaryotes and this diversification of function could account for the evolutionary conservation of duplicated Argonaute-Piwi proteins. In contrast, additional RNAi-mediated pathways such as RNA-directed DNA methylation, programmed genome rearrangements, meiotic silencing by unpaired DNA, and miRNA-mediated gene regulation may have evolved independently in specific lineages.

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Section: Phytophthora Infestansmentioning

confidence: 99%

Section: Phytophthora Infestansmentioning

confidence: 99%

On the origin and functions of RNA-mediated silencing: from protists to man

2006

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“…Both constructs were transformed into wild-type cells. In the following section, we present data that were obtained with the RNAi construct designed according to the method described by Rohr et al (2004) due to its higher stability compared to the classical RNAi approach. Nevertheless, both RNAi approaches showed similar results.…”

Section: Generation and Characterization Of An Rnai Knockdown Strainmentioning

confidence: 99%

“…A classical RNAi construct, using the expression vector pCB740 (Schroda et al, 1999) with 440 bp of the 5¢ coding sequence of ferritin in the antisense orientation, was generated. The second RNAi construct contained a cassette consisting of 410 bp of the coding region of ferritin in antisense orientation separated by a 310-bp long spacer and was inserted in the RNAi vector designed by Rohr et al (2004). Both constructs were transformed into wild-type cells.…”

Section: Generation and Characterization Of An Rnai Knockdown Strainmentioning

confidence: 99%

“…Its ability to grow photo-heterotrophically or photo-autotrophically, the possibility of transforming all three genomes (Rochaix, 1995), all of which are sequenced (Maul et al, 2002;Merchant et al, 2007;Michaelis et al, 1990), and numerous molecular tools such as RNAi (Rohr et al, 2004) as well as proteomic approaches (Hippler et al, 2001) make Chlamydomonas a versatile model organism. Numerous studies have been published with respect to its iron homeostasis and consequences of iron deficiency (Allen et al, 2007;La Fontaine et al, 2002;Moseley et al, 2002;Naumann et al, 2005Naumann et al, , 2007, showing that Chlamydomonas reacts in a fine-tuned manner to changing iron availability.…”

Section: Introductionmentioning

confidence: 99%

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Ferritin is required for rapid remodeling of the photosynthetic apparatus and minimizes photo‐oxidative stress in response to iron availability in Chlamydomonas reinhardtii

et al. 2008

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SummaryFerritin is a key player in the iron homeostasis due to its ability to store large quantities of iron. Chlamydomonas reinhardtii contains two nuclear genes for ferritin (ferr1 and ferr2) that are induced when Chlamydomonas cells are shifted to iron-deficient conditions. In response to the reduced iron availability, degradation of photosystem I (PSI) and remodeling of its light-harvesting complex occur. This active PSI degradation slows down under photo-autotrophic conditions where photosynthesis is indispensable. We observed a strong induction of ferritin correlated with the degree of PSI degradation during iron deficiency. The PSI level can be restored to normal within 24 h after iron repletion at the expense of the accumulated ferritin, indicating that the ferritin-stored iron allows fast adjustment of the photosynthetic apparatus with respect to iron availability. RNAi strains that are significantly reduced in the amount of ferritin show a striking delay in the degradation of PSI under iron deficiency. Furthermore, these strains are more susceptible to photo-oxidative stress under high-light conditions. We conclude that (i) ferritin is used to buffer the iron released by degradation of the photosynthetic complexes, (ii) the physiological status of the cell determines the strategy used to overcome the impact of iron deficiency, (iii) the availability of ferritin is important for rapid degradation of PSI under iron deficiency, and (iv) ferritin plays a protective role under photo-oxidative stress conditions.

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Successful reversal of transgene silencing in Chlamydomonas reinhardtii

Beauchemin,

Merindol,

Fantino

et al. 2023

Biotechnology Journal

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Chlamydomonas reinhardtii has been successfully engineered to produce compounds of interest following transgene integration and heterologous protein expression. The advantages of this model include the availability of validated tools for bioengineering, its photosynthetic ability, and its potential use as biofuel. Despite this, breakthroughs have been hindered by its ability to silence transgene expression through epigenetic changes. Histone deacetylases (HDAC) are main players in gene expression. We hypothesized that transgene silencing can be reverted with chemical treatments using HDAC inhibitors. To analyze this, we transformed C. reinhardtii, integrating into its genome the mVenus reporter gene under the HSP70‐rbcs2 promoter. From 384 transformed clones, 88 (22.9%) displayed mVenus positive (mVenus+) cells upon flow‐cytometry analysis. Five clones with different fluorescence intensities were selected. The number of integrated copies was measured by qPCR. Transgene expression levels were followed over the growth cycle and upon SAHA treatment, using a microplate reader, flow cytometry, RT‐qPCR, and western blot analysis. First, we observed that expression varies with the cell cycle, reaching a maximum level just before the stationary phase in all clones. Second, we uncovered that supplementation with HDAC inhibitors of the hydroxamate family, such as vorinostat (suberoylanilide‐hydroxamic‐acid, SAHA) at the initiation of culture increases the frequency (% of mVenus+ cells) and the level of transgene expression per cell over the whole growth cycle, through histone deacetylase inhibition. Thus, we propose a new tool to successfully trigger the expression of heterologous proteins in the green algae C. reinhardtii, overcoming its main obstacle as an expression platform.This article is protected by copyright. All rights reserved

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Tandem inverted repeat system for selection of effective transgenic RNAi strains in Chlamydomonas

Cited by 150 publications

References 73 publications

On the origin and functions of RNA-mediated silencing: from protists to man

On the origin and functions of RNA-mediated silencing: from protists to man

Ferritin is required for rapid remodeling of the photosynthetic apparatus and minimizes photo‐oxidative stress in response to iron availability in Chlamydomonas reinhardtii

Successful reversal of transgene silencing in Chlamydomonas reinhardtii

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