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Targeting a heterologous protein to multiple plant organelles via rationally designed 5′ mRNA tags

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2013

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BioMed Central
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Voges, Mathias J, Pamela A Silver, Jeffrey C Way, and Matthew D Mattozzi. 2013. “Targeting a heterologous protein to multiple plant organelles via rationally designed 5′ mRNA tags.” Journal of Biological Engineering 7 (1): 20. doi:10.1186/1754-1611-7-20. http://dx.doi.org/10.1186/1754-1611-7-20.

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Abstract

Background: Plant bioengineers require simple genetic devices for predictable localization of heterologous proteins to multiple subcellular compartments. Results: We designed novel hybrid signal sequences for multiple-compartment localization and characterize their function when fused to GFP in Nicotiana benthamiana leaf tissue. TriTag-1 and TriTag-2 use alternative splicing to generate differentially localized GFP isoforms, localizing it to the chloroplasts, peroxisomes and cytosol. TriTag-1 shows a bias for targeting the chloroplast envelope while TriTag-2 preferentially targets the peroxisomes. TriTag-3 embeds a conserved peroxisomal targeting signal within a chloroplast transit peptide, directing GFP to the chloroplasts and peroxisomes. Conclusions: Our novel signal sequences can reduce the number of cloning steps and the amount of genetic material required to target a heterologous protein to multiple locations in plant cells. This work harnesses alternative splicing and signal embedding for engineering plants to express multi-functional proteins from single genetic constructs.

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Protein targeting, Alternative splicing, Signal embedding, Localization, Peroxisome, Chloroplast, Cytosol, Organelle,

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