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High-level expression of thermostable cellulolytic enzymes in tobacco transplastomic plants and their use in hydrolysis of an industrially pretreated Arundo donax L. biomass

Biotechnology for Biofuels (2016) 9(1)
DOI: 10.1186/s13068-016-0569-z
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Abstract

Background: Biofuels production from plant biomasses is a complex multi-step process with important economic burdens. Several biotechnological approaches have been pursued to reduce biofuels production costs. The aim of the present study was to explore the production in tobacco plastome of three genes encoding (hemi)cellulolytic enzymes from thermophilic and hyperthermophilic bacterium and Archaea, respectively, and test their application in the bioconversion of an important industrially pretreated biomass feedstock (A. donax) for production of second-generation biofuels. Results: The selected enzymes, endoglucanase, endo-β-1,4-xylanase and β-glucosidase, were expressed in tobacco plastome with a protein yield range from 2 % to more than 75 % of total soluble proteins (TSP). The accumulation of endoglucanase (up to 2 % TSP) gave altered plant phenotypes whose severity was directly linked to the enzyme yield. The most severe seedling-lethal phenotype was due to the impairment of plastid development associated to the binding of endoglucanase protein to thylakoids. Endo-β-1,4-xylanase and β-glucosidase, produced at very high level without detrimental effects on plant development, were enriched (fourfold) by heat treatment (105.4 and 255.4 U/mg, respectively). Both plastid-derived biocatalysts retained the main features of the native or recombinantly expressed enzymes with interesting differences. Plastid-derived xylanase and β-glucosidase resulted more thermophilic than the E. coli recombinant and native counterpart, respectively. Bioconversion experiments, carried out at 50 and 60 °C, demonstrated that plastid-derived enzymes were able to hydrolyse an industrially pretreated giant reed biomass. In particular, the replacement of commercial enzyme with plastid-derived xylanase, at 60 °C, produced an increase of both xylose recovery and hydrolysis rate; whereas the replacement of both xylanase and β-glucosidase produced glucose levels similar to those observed with the commercial cocktails, and xylose yields always higher in the whole 24-72 h range. Conclusions: The very high production level of thermophilic and hyperthermophilic enzymes, their stability and bioconversion efficiencies described in this study demonstrate that plastid transformation represents a real cost-effective production platform for cellulolytic enzymes.

Figures

  • Fig. 1 Plastid vectors and expression cassettes used in transformation experiments, containing transgenes encoding cellulolytic enzymes. For each vectors, regulatory sequences, protein accumulation level and phenotype in corresponding transplastomic plants are indicated
  • Fig. 2 Southern blot analyses of plastid transformants to select independently generated homoplasmic lines per each construct. Schematic rep‑ resentation of the targeting region in the plastid genome (Nt‑ptDNA) and maps of transformed (Nt‑DC series) plastid genome regions involved in transgene integration (a). Lines with the same number but different letters indicate transplastomic lines generated from the same primary shoot. For DC11 and DC21 transplastomic plants, heteroplasmic lines (marked with an asterisk) containing both wild‑type and transformed plastomes are also shown (b). Below the maps are indicated the expected sizes of the BamHI DNA fragments in Southern blot analyses. rps12/7 and trnV correspond to the plastome integration site of the expression cassettes; aadA, aminoglycoside 3′ adenylyltransferase marker gene
  • Fig. 3 Plant phenotypes. Comparison of plant growth between mature control (PH and PRV, wild‑type and transformed with the empty vector, respectively) and transplastomic plants expressing endoglucanase (DC1, DC2 and DC3), endo‑β‑1,4‑xylanase (DC11) and β‑glucosidase (DC21 and DC23) cellulolytic enzymes under photoautotrophic conditions in soil
  • Fig. 4 Detection by Western blot analysis of cellulolytic enzymes accumulated in transplastomic DC plants. Each transplastomic line shows a prominent additional protein band corresponding in size to the foreign protein. Endoglucanase (a) and endo‑β‑1,4‑xylanase (b) enzymes accumulation in DC1, DC2, DC3 and DC11 transplastomic plants, respectively (T1 generation). c Accumulation of β‑glucosidase enzyme in DC21 and DC23 transplastomic plants (T0 generation). FLAG: recombinant Flag standard protein; PRV: transplastomic control plant transformed with the empty vector
  • Fig. 5 Detection by Coomassie blue staining of polyacrylamide gel of cellulolytic enzymes accumulated in transplastomic DC plants. Each leaf of different age of transplastomic line shows a prominent additional protein band corresponding in size to the foreign protein. DC11 T1 transplastomic plants expressing endo‑β‑1,4‑xylanase (xyn), DC21, DC23 T0 transplastomic plants expressing β‑glucosidase (celB), PH wild‑type plant. 1 young leaf; 2 mature leaf; 3 old leaf; RbcL Rubisco large subunit protein
  • Fig. 6 Transmission Electron Microscopy (TEM) images of cells and plastids of control and endoglucanase‑expressing transplastomic plants. PRV control plants (a) show mature chloroplasts, whereas for endoglucanase‑expressing transplastomic plants the coexistence of mature chloroplast and plastid resembling proplastid in DC1 plants (b) and the prevalent presence of proplastids containing vesicles in DC2 (c) and DC3 (d) plants were observed. Arrows in a and b indicate grana and inter‑grana structures. Arrowheads in c and d point to rudimentary thylakoids. Ch chloroplast, cw cell wall, p plastid, m mitochondria, g plastoglobules, v vesicles. Scale bars 100 nm
  • Fig. 7 Sub‑organellar localization of endoglucanase. Western blot analyses of chloroplast subfractions from control (PRV) and endoglu‑ canase (DC2) transplastomic plants performed using monoclonal and polyclonal antibodies raised against Flag tag, RbcL (stroma marker) and D1 (thylakoid marker). Tc total chloroplast proteins, S stroma proteins, T thylakoid proteins
  • Table 1 Enzyme yield in transplastomic tobacco plants and partial purification of plastid-based cellulolytic enzymes

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APA

Castiglia, D., Sannino, L., Marcolongo, L., Ionata, E., Tamburino, R., De Stradis, A., … Scotti, N. (2016). High-level expression of thermostable cellulolytic enzymes in tobacco transplastomic plants and their use in hydrolysis of an industrially pretreated Arundo donax L. biomass. Biotechnology for Biofuels, 9(1). https://doi.org/10.1186/s13068-016-0569-z

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