Showing papers by "Pal Maliga published in 2019"
TL;DR: A study used engineered, nuclear-expressed pentatricopeptide repeat proteins with programmable RNA sequence specificity to boost the expression of chloroplast transgenes harbouring cognate cis-elements, providing a method for regulating plastid transgene expression.
Abstract: The engineering of plant genomes presents exciting opportunities to modify agronomic traits and to produce high-value products in plants. Expression of foreign proteins from transgenes in the chloroplast genome offers advantages that include the capacity for prodigious protein output, the lack of transgene silencing and the ability to express multicomponent pathways from polycistronic mRNA. However, there remains a need for robust methods to regulate plastid transgene expression. We designed orthogonal activators that boost the expression of chloroplast transgenes harbouring cognate cis-elements. Our system exploits the programmable RNA sequence specificity of pentatricopeptide repeat proteins and their native functions as activators of chloroplast gene expression. When expressed from nuclear transgenes, the engineered proteins stimulate the expression of plastid transgenes by up to ~40-fold, with maximal protein abundance approaching that of Rubisco. This strategy provides a means to regulate and optimize the expression of foreign genes in chloroplasts and to avoid deleterious effects of their products on plant growth. A study used engineered, nuclear-expressed pentatricopeptide repeat proteins with programmable RNA sequence specificity to boost the expression of chloroplast transgenes harbouring cognate cis-elements, providing a method for regulating plastid transgene expression.
39 citations
TL;DR: A regulatory system comprising a variant of the maize RNA-binding protein PPR10 and a cognate binding site upstream of a plastid transgene that encodes green fluorescent protein (GFP) enables an increase inTransgene expression in non-photosynthetic plastids without interfering with chloroplast gene expression in leaves.
Abstract: Non-green plastids are desirable for the expression of recombinant proteins in edible plant parts to enhance the nutritional value of tubers or fruits, or to deliver pharmaceuticals. However, plastid transgenes are expressed at extremely low levels in the amyloplasts of storage organs such as tubers1-3. Here, we report a regulatory system comprising a variant of the maize RNA-binding protein PPR10 and a cognate binding site upstream of a plastid transgene that encodes green fluorescent protein (GFP). The binding site is not recognized by the resident potato PPR10 protein, restricting GFP protein accumulation to low levels in leaves. When the PPR10 variant is expressed from the tuber-specific patatin promoter, GFP accumulates up to 1.3% of the total soluble protein, a 60-fold increase compared with previous studies2 (0.02%). This regulatory system enables an increase in transgene expression in non-photosynthetic plastids without interfering with chloroplast gene expression in leaves.
27 citations
TL;DR: New transformation-competent Arabidopsis lines, with new plastid transformation vectors and a protocol for measuring plastsid transformation efficiency, will advance the engineering of the plASTid genome in Arabidoptera.
Abstract: New transformation-competent Arabidopsis lines, with new plastid transformation vectors and a protocol for measuring plastid transformation efficiency, will advance the engineering of the plastid genome in Arabidopsis.
10 citations