The stem-loop region of the tobacco  psbA 5′UTR is an important determinant of mRNA stability and translation efficiency

Zou, Zhurong; Eibl, Christian; Koop, Hans‐Ulrich

doi:10.1007/s00438-003-0842-2

Cited by 95 publications

(79 citation statements)

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“…Among more than 150 transgenes expressed in chloroplasts, more than 75% utilized psbA regulatory sequences (Jin and Daniell, 2015;Daniell et al, 2016aDaniell et al, , 2016b. In addition, three ribosome-binding regions in the 5ʹ UTR of psbA recruit ribosomes and efficiently form the translational initiation complex (Zou et al, 2003). Therefore, it is expected that improvement of translation elongation in heterologous genes should increase transgene expression.…”

Section: Discussionmentioning

confidence: 99%

Codon Optimization to Enhance Expression Yields Insights into Chloroplast Translation

et al. 2016

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Codon optimization based on psbA genes from 133 plant species eliminated 105 (human clotting factor VIII heavy chain [FVIII HC]) and 59 (polio VIRAL CAPSID PROTEIN1 [VP1]) rare codons; replacement with only the most highly preferred codons decreased transgene expression (77-to 111-fold) when compared with the codon usage hierarchy of the psbA genes. Targeted proteomic quantification by parallel reaction monitoring analysis showed 4.9-to 7.1-fold or 22.5-to 28.1-fold increase in FVIII or VP1 codon-optimized genes when normalized with stable isotope-labeled standard peptides (or housekeeping protein peptides), but quantitation using western blots showed 6.3-to 8-fold or 91-to 125-fold increase of transgene expression from the same batch of materials, due to limitations in quantitative protein transfer, denaturation, solubility, or stability. Parallel reaction monitoring, to our knowledge validated here for the first time for in planta quantitation of biopharmaceuticals, is especially useful for insoluble or multimeric proteins required for oral drug delivery. Northern blots confirmed that the increase of codonoptimized protein synthesis is at the translational level rather than any impact on transcript abundance. Ribosome footprints did not increase proportionately with VP1 translation or even decreased after FVIII codon optimization but is useful in diagnosing additional rate-limiting steps. A major ribosome pause at CTC leucine codons in the native gene of FVIII HC was eliminated upon codon optimization. Ribosome stalls observed at clusters of serine codons in the codon-optimized VP1 gene provide an opportunity for further optimization. In addition to increasing our understanding of chloroplast translation, these new tools should help to advance this concept toward human clinical studies.

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Section: Discussionmentioning

confidence: 99%

Codon Optimization to Enhance Expression Yields Insights into Chloroplast Translation

et al. 2016

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“…For supertransformation, a modified Drps15 vector was built that contained the kanamycin resistance gene aphA-6 instead of the spectinomycin resistance gene aadA (Bateman and Purton, 2000;Huang et al, 2002;Fleischmann et al, 2011). The aphA-6 expression cassette was driven by the psbA promoter from Chlamydomonas reinhardtii and the rbcL 39 untranslated region from C. reinhardtii (Zou et al, 2003). The cassette was excised with SmaI and inserted into a unique HincII restriction site in the rps15 coding region (Fleischmann et al, 2011;Figure 1).…”

Section: Construction Of Plastid Transformation Vectorsmentioning

confidence: 99%

Synthetic Lethality in the Tobacco Plastid Ribosome and Its Rescue at Elevated Growth Temperatures

et al. 2014

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ORCID ID: 0000-0001-7502-6940 (R.B.)Consistent with their origin from cyanobacteria, plastids (chloroplasts) perform protein biosynthesis on bacterial-type 70S ribosomes. The plastid genomes of seed plants contain a conserved set of ribosomal protein genes. Three of these have proven to be nonessential for translation and, thus, for cellular viability: rps15, rpl33, and rpl36. To help define the minimum ribosome, here, we examined whether more than one of these nonessential plastid ribosomal proteins can be removed from the 70S ribosome. To that end, we constructed all possible double knockouts for the S15, L33, and L36 ribosomal proteins by stable transformation of the tobacco (Nicotiana tabacum) plastid genome. We find that, although S15 and L33 function in different ribosomal particles (30S and 50S, respectively), their combined deletion from the plastid genome results in synthetic lethality under autotrophic conditions. Interestingly, the lethality can be overcome by growth under elevated temperatures due to an improved efficiency of plastid ribosome biogenesis. Our results reveal functional interactions between protein and RNA components of the 70S ribosome and uncover the interdependence of the biogenesis of the two ribosomal subunits. In addition, our findings suggest that defining a minimal set of plastid genes may prove more complex than generally believed.

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“…Rather, alternative codons may affect the tertiary structure of mRNA, thereby affecting mRNA degradation rate, mRNA half-life, and hence the rate of protein expression. 30 …”

Section: Functional Pseudogenesmentioning

confidence: 99%

Expanding the ‘central dogma’: the regulatory role of nonprotein coding genes and implications for the genetic liability to schizophrenia

2004

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The stem-loop region of the tobacco psbA 5′UTR is an important determinant of mRNA stability and translation efficiency

Cited by 95 publications

References 50 publications

Codon Optimization to Enhance Expression Yields Insights into Chloroplast Translation

Codon Optimization to Enhance Expression Yields Insights into Chloroplast Translation

Synthetic Lethality in the Tobacco Plastid Ribosome and Its Rescue at Elevated Growth Temperatures

Expanding the ‘central dogma’: the regulatory role of nonprotein coding genes and implications for the genetic liability to schizophrenia

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