Cinnamoyl-CoA reductase explained

cinnamoyl-CoA reductase
Ec Number:1.2.1.44
Cas Number:59929-39-4
Go Code:0016621
Cinnamoyl-CoA reductase

Cinnamoyl-CoA reductase, systematically named cinnamaldehyde:NADP+ oxidoreductase (CoA-cinnamoylating) but commonly referred to by the acronym CCR, is an enzyme that catalyzes the reduction of a substituted cinnamoyl-CoA to its corresponding cinnamaldehyde, utilizing NADPH and H+ and releasing free CoA and NADP+ in the process.[1] Common biologically relevant cinnamoyl-CoA substrates for CCR include p-coumaroyl-CoA and feruloyl-CoA, which are converted into p-coumaraldehyde and coniferaldehyde, respectively,[2] though most CCRs show activity toward a variety of other substituted cinnamoyl-CoA's as well. Catalyzing the first committed step in monolignol biosynthesis,[3] this enzyme plays a critical role in lignin formation, a process important in plants both for structural development and defense response.

Structure

The first confirmed CCR was isolated from soybean (Glycine max) in 1976.[4] However, crystal structures have so far been reported for just three CCR homologs: Petunia x hybrida CCR1, Medicago truncatula CCR2, and Sorghum bicolor CCR1.[5] While the enzyme crystallizes as an asymmetric dimer, it is thought to exist as a monomer in the cytoplasm, with each individual protein having a bilobal structure consisting of two domains surrounding a large, empty inner cleft for substrate binding. Typical CCRs have a molecular weight of around 36-38 kDa.

The domain containing the enzyme's N-terminus consists of several alpha helices and six beta strands that, in addition to a seventh strand connected to the C-terminus side of the enzyme, form a parallel beta sheet structure known as a Rossmann fold. In CCR, this fold structure, a common motif amongst proteins, serves as a binding domain for NADPH. The second domain, which consists of several alpha helices, beta strands, and extended loops, is responsible for binding the cinnamoyl-CoA substrate. These two domains are situated in such a way that the binding sites for NADPH and cinnamoyl-CoA are positioned closely to one another at the lobes' interface.

Though attempts to cocrystallize the enzyme with a bound cinnamoyl-CoA have thus far been unsuccessful, molecular docking studies indicate that the CoA segment of these molecules folds around to bind along the outer part of the inter-domain cleft, while the phenyl-containing portion of these substrates likely binds in the deepest part of the cleft. This inner part of the pocket contains several amino acids with nonpolar side chains necessary for stabilization of the hydrophobic phenyl ring in addition to a tyrosine residue important for hydrogen bond formation with the ring's 4-hydroxyl group. The particular identities of the nonpolar residues are believed to play a critical role in determining substrate specificity.

Mechanism

The mechanism for the reduction of the CoA thioester to the aldehyde involves a hydride transfer to the carbonyl carbon from NADPH, forming a tetrahedral intermediate with a formal negative charge on the oxygen atom. This negative charge is thought to be stabilized partially via hydrogen bonding with the hydrogen atoms of nearby tyrosine and serine side chains. The serine and tyrosine residues are conserved across all CCRs as part of a catalytic triad along with lysine, which is thought to control the pKa of the tyrosine via electrostatic interactions with the ribose group of the NADPH.

The tetrahedral intermediate then collapses, kicking out the CoA and forming an aldehyde as the final product. The thiolate of the CoA is protonated either as it leaves by a nearby residue or after it is free from the binding pocket and out of the enzyme all-together; the exact mechanism is currently unclear, but evidence suggests that a cysteine residue may play the role of thiolate proton donor.

Biological Function

Phylogenomic analysis indicates that enzymes with true CCR activity first evolved in the of land plants. Most if not all modern land plants and all vascular plants are believed to have at least one functional CCR, an absolute requirement for any plant species with lignified tissues.[6] Most CCR homologs are highly expressed during development, especially in stem, root, and xylem cells which require the enhanced structural support provided by lignin. However, certain CCRs are not constitutively expressed throughout development and are only up-regulated during enhanced lignification in response to stressors such as pathogen attack. CCR is especially important because it acts as a final control point for regulation of metabolic flux toward the monolignols and therefore toward lignin as well;[7] prior to this reduction step, the cinnamoyl-CoA's can still enter into other expansive specialized metabolic pathways. For example, feruloyl-CoA is a precursor of the coumarin scopoletin,[8] a compound believed to play an important role in plant pathogen response.[9] CCR also plays a role in determining lignin composition by regulating levels of the different monomers according to its specific activity toward particular cinnamoyl-CoA's. Monocots and dicots, for example, tend to have very different lignin patterns: lignin found in monocots typically has a higher percentage of p-coumaroyl alcohol-derived subunits, while lignin found in dicots is typically composed of almost entirely coniferyl alcohol and sinapyl alcohol subunits. As can be seen in the diagram shown to the right, these monolignols are derived directly from their corresponding aldehydes, except in the case of sinapyl alcohol - while several CCR homologs have been shown to act on sinapoyl-CoA in vitro, it is unclear whether this activity is biologically relevant and most current models of the lignin pathway do not include this reaction as a valid step.[10]

Recent studies indicate that many plant species have two distinct homologs of CCR with differential activity in planta. In some plants the two homologs vary primarily by substrate specificity. For example, CCR1 of the model legume Medicago truncatula shows strong preference toward feruloyl-CoA (typical of most CCRs), while the plant's CCR2 exhibits a clear preference for both p-coumaroyl- and caffeoyl-CoA. This second CCR, which is allosterically activated by its preferred substrates but inhibited by feruloyl-CoA, is thought to act as part of a shunt pathway toward coniferaldehyde that enhances the pathway's overall flexibility and robustness in different conditions.[11] In other cases though, the two homologs vary primarily by expression pattern. In the model plant Arabidopsis thaliana, for instance, the CCR1 and CCR2 homologs both display higher activity toward feruloyl-CoA than other substrates, but CCR2 is only expressed transiently during bacterial infection. The homolog pair in switchgrass (Panicum virgatum) differs in both ways: CCR2 prefers p-coumaroyl- and caffeoyl-CoA and is only expressed under specifically induced conditions, while CCR1 prefers feruloyl-CoA and is expressed constitutively in lignifying tissue.[12]

Regulation of CCR expression is thought to occur primarily at the transcriptional level. In Arabidopsis thaliana, several of the required transcription factors for CCR expression have actually been identified, including MYB58 and MYB63, both of which are implicated generally in secondary cell wall formation. It has been shown that over-expression of these two transcription factors results in a 2- to 3-fold increase in CCR mRNA transcripts, though intriguingly, the up-regulation of genes further upstream in the monolignol pathway is even greater.[13] Non-transcriptional regulation of CCR, however, can be important as well. In rice (Oryza sativa), for example, evidence suggests that the CCR1 homolog is an effector of Rac1, a small GTPase important for plant defense response. In this case, the Rac1 protein is proposed to activate CCR upon binding, leading to enhanced monolignol biosynthesis. Because Rac1 also activates NADPH oxidase, which produces peroxides critical for monolignol polymerization, overall lignin biosynthesis is enhanced as well.[14]

Biotechnological significance

Efforts to engineer plant cell wall formation for enhanced biofuel production commonly target lignin biosynthesis in order to reduce lignin content and thereby improve yields of ethanol from cellulose, a complex polysaccharide important for cell wall structure.[15] Lignin is troublesome for biofuel production because it is the main contributor to plant biomass recalcitrance due to its toughness and heterogeneity. By reducing lignin content, the cellulose is more easily accessible to the chemical and biological reagents used to break it down.[16] Lowering the expression level of CCR in particular has emerged as a common strategy for accomplishing this goal, and this strategy has resulted in successful lignin content reduction and increased ethanol production from several plant species including tobacco (Nicotiana tabacum)[3] and poplar (Populus tremula x Populus alba). Challenges with this strategy include the wide variation in expression levels associated with current plant genetic transformation technologies in addition to the dramatic decrease in overall growth and biomass that typically accompanies low lignin production. However, it has been shown that by targeting CCR down-regulation to specific tissue types[17] or coupling it to down-regulation of cinnamyl alcohol dehydrogenase (CAD),[18] the latter challenge at least can be somewhat mitigated.

Notes and References

  1. Pan H, Zhou R, Louie GV, Mühlemann JK, Bomati EK, Bowman ME, Dudareva N, Dixon RA, Noel JP, Wang X . Structural studies of cinnamoyl-CoA reductase and cinnamyl-alcohol dehydrogenase, key enzymes of monolignol biosynthesis . The Plant Cell . 26 . 9 . 3709–27 . September 2014 . 25217505 . 4213152 . 10.1105/tpc.114.127399 .
  2. Barros J, Serk H, Granlund I, Pesquet E . The cell biology of lignification in higher plants . Annals of Botany . 115 . 7 . 1053–74 . June 2015 . 25878140 . 4648457 . 10.1093/aob/mcv046 .
  3. Lauvergeat V, Lacomme C, Lacombe E, Lasserre E, Roby D, Grima-Pettenati J . Two cinnamoyl-CoA reductase (CCR) genes from Arabidopsis thaliana are differentially expressed during development and in response to infection with pathogenic bacteria . Phytochemistry . 57 . 7 . 1187–95 . August 2001 . 11430991 . 10.1016/s0031-9422(01)00053-x .
  4. Wengenmayer H, Ebel J, Grisebach H . Enzymic synthesis of lignin precursors. Purification and properties of a cinnamoyl-CoA: NADPH reductase from cell suspension cultures of soybean (Glycinemax) . European Journal of Biochemistry . 65 . 2 . 529–36 . June 1976 . 7454 . 10.1111/j.1432-1033.1976.tb10370.x . free .
  5. Sattler SA, Walker AM, Vermerris W, Sattler SE, Kang C . Structural and Biochemical Characterization of Cinnamoyl-CoA Reductases . Plant Physiology . 173 . 2 . 1031–1044 . February 2017 . 27956488 . 5291045 . 10.1104/pp.16.01671 .
  6. Barakat A, Yassin NB, Park JS, Choi A, Herr J, Carlson JE . Comparative and phylogenomic analyses of cinnamoyl-CoA reductase and cinnamoyl-CoA-reductase-like gene family in land plants . Plant Science . 181 . 3 . 249–57 . September 2011 . 21763535 . 10.1016/j.plantsci.2011.05.012 .
  7. Ma QH, Tian B . Biochemical characterization of a cinnamoyl-CoA reductase from wheat . Biological Chemistry . 386 . 6 . 553–60 . June 2005 . 16006242 . 10.1515/BC.2005.065 . 12173262 .
  8. Kai K, Mizutani M, Kawamura N, Yamamoto R, Tamai M, Yamaguchi H, Sakata K, Shimizu B . Scopoletin is biosynthesized via ortho-hydroxylation of feruloyl CoA by a 2-oxoglutarate-dependent dioxygenase in Arabidopsis thaliana . The Plant Journal . 55 . 6 . 989–99 . September 2008 . 18547395 . 10.1111/j.1365-313X.2008.03568.x . free .
  9. Sun H, Wang L, Zhang B, Ma J, Hettenhausen C, Cao G, Sun G, Wu J, Wu J . Scopoletin is a phytoalexin against Alternaria alternata in wild tobacco dependent on jasmonate signalling . Journal of Experimental Botany . 65 . 15 . 4305–15 . August 2014 . 24821958 . 4112635 . 10.1093/jxb/eru203 .
  10. Vanholme R, Demedts B, Morreel K, Ralph J, Boerjan W . Lignin biosynthesis and structure . Plant Physiology . 153 . 3 . 895–905 . July 2010 . 20472751 . 2899938 . 10.1104/pp.110.155119 .
  11. Zhou R, Jackson L, Shadle G, Nakashima J, Temple S, Chen F, Dixon RA . Distinct cinnamoyl CoA reductases involved in parallel routes to lignin in Medicago truncatula . Proceedings of the National Academy of Sciences of the United States of America . 107 . 41 . 17803–8 . October 2010 . 20876124 . 2955080 . 10.1073/pnas.1012900107 . 2010PNAS..10717803Z . free .
  12. Escamilla-Treviño LL, Shen H, Uppalapati SR, Ray T, Tang Y, Hernandez T, Yin Y, Xu Y, Dixon RA . Switchgrass (Panicum virgatum) possesses a divergent family of cinnamoyl CoA reductases with distinct biochemical properties . The New Phytologist . 185 . 1 . 143–55 . January 2010 . 19761442 . 10.1111/j.1469-8137.2009.03018.x .
  13. Zhou J, Lee C, Zhong R, Ye ZH . MYB58 and MYB63 are transcriptional activators of the lignin biosynthetic pathway during secondary cell wall formation in Arabidopsis . The Plant Cell . 21 . 1 . 248–66 . January 2009 . 19122102 . 2648072 . 10.1105/tpc.108.063321 .
  14. Kawasaki T, Koita H, Nakatsubo T, Hasegawa K, Wakabayashi K, Takahashi H, Umemura K, Umezawa T, Shimamoto K . Cinnamoyl-CoA reductase, a key enzyme in lignin biosynthesis, is an effector of small GTPase Rac in defense signaling in rice . Proceedings of the National Academy of Sciences of the United States of America . 103 . 1 . 230–5 . January 2006 . 16380417 . 1325009 . 10.1073/pnas.0509875103 . 2006PNAS..103..230K . free .
  15. Loqué D, Scheller HV, Pauly M . Engineering of plant cell walls for enhanced biofuel production . Current Opinion in Plant Biology . 25 . 151–61 . June 2015 . 26051036 . 10.1016/j.pbi.2015.05.018 . free .
  16. Van Acker R, Leplé JC, Aerts D, Storme V, Goeminne G, Ivens B, Légée F, Lapierre C, Piens K, Van Montagu MC, Santoro N, Foster CE, Ralph J, Soetaert W, Pilate G, Boerjan W . Improved saccharification and ethanol yield from field-grown transgenic poplar deficient in cinnamoyl-CoA reductase . Proceedings of the National Academy of Sciences of the United States of America . 111 . 2 . 845–50 . January 2014 . 24379366 . 3896177 . 10.1073/pnas.1321673111 . 2014PNAS..111..845V . free .
  17. Smith RA, Schuetz M, Roach M, Mansfield SD, Ellis B, Samuels L . Neighboring parenchyma cells contribute to Arabidopsis xylem lignification, while lignification of interfascicular fibers is cell autonomous . The Plant Cell . 25 . 10 . 3988–99 . October 2013 . 24096341 . 3877792 . 10.1105/tpc.113.117176 .
  18. Chabannes M, Barakate A, Lapierre C, Marita JM, Ralph J, Pean M, Danoun S, Halpin C, Grima-Pettenati J, Boudet AM . Strong decrease in lignin content without significant alteration of plant development is induced by simultaneous down-regulation of cinnamoyl CoA reductase (CCR) and cinnamyl alcohol dehydrogenase (CAD) in tobacco plants . The Plant Journal . 28 . 3 . 257–70 . November 2001 . 11722769 . 10.1046/j.1365-313x.2001.01140.x . free .