Determining the Rate-Limiting Step for Light-Responsive Redox Regulation in Chloroplasts

Thiol-based redox regulation ensures light-responsive control of chloroplast functions. Light-derived signal is transferred in the form of reducing power from the photosynthetic electron transport chain to several redox-sensitive target proteins. Two types of protein, ferredoxin-thioredoxin reductase (FTR) and thioredoxin (Trx), are well recognized as the mediators of reducing power. However, it remains unclear which step in a series of redox-relay reactions is the critical bottleneck for determining the rate of target protein reduction. To address this, the redox behaviors of FTR, Trx, and target proteins were extensively characterized in vitro and in vivo. The FTR/Trx redox cascade was reconstituted in vitro using recombinant proteins from Arabidopsis. On the basis of this assay, we found that the FTR catalytic subunit and f-type Trx are rapidly reduced after the drive of reducing power transfer, irrespective of the presence or absence of their downstream target proteins. By contrast, three target proteins, fructose 1,6-bisphosphatase (FBPase), sedoheptulose 1,7-bisphosphatase (SBPase), and Rubisco activase (RCA) showed different reduction patterns; in particular, SBPase was reduced at a low rate. The in vivo study using Arabidopsis plants showed that the Trx family is commonly and rapidly reduced upon high light irradiation, whereas FBPase, SBPase, and RCA are differentially and slowly reduced. Both of these biochemical and physiological findings suggest that reducing power transfer from Trx to its target proteins is a rate-limiting step for chloroplast redox regulation, conferring distinct light-responsive redox behaviors on each of the targets.

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The rate-limiting step of protein synthesis in vivo and in vitro and the distribution of growing peptides between the puromycinlabile and puromycin-non-labile sites on polyribosomes

Biochemical Journal ◽

10.1042/bj1220267 ◽

1971 ◽

Vol 122 (3) ◽

pp. 267-276 ◽

Cited By ~ 10

Author(s):

D. C. N. Earl ◽

Susan T. Hindley

Keyword(s):

Amino Acids ◽

Protein Synthesis ◽

Donor Site ◽

Peptide Bond ◽

Rate Limiting Step ◽

Limiting Step ◽

Donor And Acceptor ◽

Rate Limiting

1. At 3 min after an intravenous injection of radioactive amino acids into the rat, the bulk of radioactivity associated with liver polyribosomes can be interpreted as growing peptides. 2. In an attempt to identify the rate-limiting step of protein synthesis in vivo and in vitro, use was made of the action of puromycin at 0°C, in releasing growing peptides only from the donor site, to study the distribution of growing peptides between the donor and acceptor sites. 3. Evidence is presented that all growing peptides in a population of liver polyribosomes labelled in vivo are similarly distributed between the donor and acceptor sites, and that the proportion released by puromycin is not an artifact of methodology. 4. The proportion released by puromycin is about 50% for both liver and muscle polyribosomes labelled in vivo, suggesting that neither the availability nor binding of aminoacyl-tRNA nor peptide bond synthesis nor translocation can limit the rate of protein synthesis in vivo. Attempts to alter this by starvation, hypophysectomy, growth hormone, alloxan, insulin and partial hepatectomy were unsuccessful. 5. Growing peptides on liver polyribosomes labelled in a cell-free system in vitro or by incubating hemidiaphragms in vitro were largely in the donor site, suggesting that either the availability or binding of aminoacyl-tRNA, or peptide bond synthesis, must be rate limiting in vitro and that the rate-limiting step differs from that in vivo. 6. Neither in vivo nor in the hemidiaphragm system in vitro was a correlation found between the proportion of growing peptides in the donor site and changes in the rate of incorporation of radioactivity into protein. This could indicate that the intracellular concentration of amino acids or aminoacyl-tRNA limits the rate of protein synthesis and that the increased incorporation results from a rise to a higher but still suboptimum concentration.

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Coassembly of SecYEG and SecA Fully Restores the Properties of the Native Translocon

Journal of Bacteriology ◽

10.1128/jb.00493-18 ◽

2018 ◽

Vol 201 (1) ◽

Cited By ~ 8

Author(s):

Priya Bariya ◽

Linda L. Randall

Keyword(s):

Lipid Bilayers ◽

Rate Constant ◽

Apparent Rate Constant ◽

Membrane Vesicles ◽

Rate Limiting Step ◽

Limiting Step ◽

Secretory System ◽

Rate Limiting

ABSTRACTIn all cells, a highly conserved channel transports proteins across membranes. InEscherichia coli, that channel is SecYEG. Many investigations of this protein complex have used purified SecYEG reconstituted into proteoliposomes. How faithfully do activities of reconstituted systems reflect the properties of SecYEG in the native membrane environment? We investigated by comparing threein vitrosystems: the native membrane environment of inner membrane vesicles and two methods of reconstitution. One method was the widely used reconstitution of SecYEG alone into lipid bilayers. The other was our method of coassembly of SecYEG with SecA, the ATPase of the translocase. For nine different precursor species we assessed parameters that characterize translocation: maximal amplitude of competent precursor translocated, coupling of energy to transfer, and apparent rate constant. In addition, we investigated translocation in the presence and absence of chaperone SecB. For all nine precursors, SecYEG coassembled with SecA was as active as SecYEG in native membrane for each of the parameters studied. Effects of SecB on transport of precursors faithfully mimicked observations madein vivo. From investigation of the nine different precursors, we conclude that the apparent rate constant, which reflects the step that limits the rate of translocation, is dependent on interactions with the translocon of portions of the precursors other than the leader. In addition, in some cases the rate-limiting step is altered by the presence of SecB. Candidates for the rate-limiting step that are consistent with our data are discussed.IMPORTANCEThis work presents a comprehensive quantification of the parameters of transport by the Sec general secretory system in the threein vitrosystems. The standard reconstitution used by most investigators can be enhanced to yield six times as many active translocons simply by adding SecA to SecYEG during reconstitution. This robust system faithfully reflects the properties of translocation in native membrane vesicles. We have expanded the number of precursors studied to nine. This has allowed us to conclude that the rate constant for translocation varies with precursor species.

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Potential Role of Intercellular Communication in the Rate-Limiting Step in Carcinogenesis

Journal of the American College of Toxicology ◽

10.3109/10915818309140689 ◽

1983 ◽

Vol 2 (3) ◽

pp. 5-22 ◽

Cited By ~ 16

Author(s):

James E. Trosko ◽

Chia-cheng Chang

Keyword(s):

Intercellular Communication ◽

Critical Mass ◽

Epidemiological Data ◽

Malignant Cell ◽

Dna Lesions ◽

Rate Limiting Step ◽

Limiting Step ◽

Rate Limiting

In order to ascertain whether there might be a scientific basis for determining practical “thresholds” for “carcinogens,” the concepts of thresholds and carcinogens were examined in the context of some current ideas on cardnogenesis. The observation that cardnogenesis seems to involve the donal expansion of a pre-malignant cell through a series of pheno-typic changes was explained by the initiation/promotion model of cardnogenesis. Unrepaired DNA lesions, acting as substrates for mutations in dividing cells, were speculated to play a role in the initiation phase of cardnogenesis (and indirectly to the promotion phase if the lesions lead to significant cell killing, forcing “compensatory hyperplasia”). Inhibition of intercellular communication, either by cell removal, cell death, growth factors or chemical promoters, was speculated to allow the donal expansion of initiated cells to reach a “critical mass.” During that donal expansion of initiated cells, additional phenotypic changes were speculated to occur during cell replication by mutational and/or epigenetic events. Therefore, it was concluded, on the basis of this model, that conditions which prevented the inhibition of intercellular communication between normal cells and the initiated cell(s) contributed to the rate limiting step of cardnogenesis. Assuming the initiation and promotion model of cardnogenesis, the classical concepts of “thresholds” and “carcinogens” were viewed as grossly inadequate because they did not symbolically represent the known determinants of the complex carcinogenic process. Unless genetic, developmental stage, tissue, nutritional, stress, life style, as well as concurrent antagonists and/or synergists, factors are known, extrapolation about the potential carcinogenicity of a given chemical from molecular, in vitro or even in vivo experiments or epidemiological data would be extremely risky. It was concluded that, at this stage of our understanding of the mech-anism(s) of carcinogenesis, attempts to determine “thresholds” for “carcinogens” naively assume “carcinogens” are the single determinants for carcinogenesis, and that all chemicals which might influence the appearance of tumors act the same way.

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The GTPase Effector Domain Sequence of the Dnm1p GTPase Regulates Self-Assembly and Controls a Rate-limiting Step in Mitochondrial Fission

Molecular Biology of the Cell ◽

10.1091/mbc.12.9.2756 ◽

2001 ◽

Vol 12 (9) ◽

pp. 2756-2766 ◽

Cited By ~ 67

Author(s):

Noelle H. Fukushima ◽

Ellen Brisch ◽

Brian R. Keegan ◽

William Bleazard ◽

Janet M. Shaw

Keyword(s):

Mitochondrial Fission ◽

Yeast Two Hybrid ◽

Effector Domain ◽

Rate Limiting Step ◽

Limiting Step ◽

Gtpase Effector Domain ◽

Rate Limiting ◽

Two Hybrid

Dnm1p belongs to a family of dynamin-related GTPases required to remodel different cellular membranes. In budding yeast, Dnm1p-containing complexes assemble on the cytoplasmic surface of the outer mitochondrial membrane at sites where mitochondrial tubules divide. Our previous genetic studies suggested that Dnm1p's GTPase activity was required for mitochondrial fission and that Dnm1p interacted with itself. In this study, we show that bacterially expressed Dnm1p can bind and hydrolyze GTP in vitro. Coimmunoprecipitation studies and yeast two-hybrid analysis suggest that Dnm1p oligomerizes in vivo. With the use of the yeast two-hybrid system, we show that this Dnm1p oligomerization is mediated, in part, by a C-terminal sequence related to the GTPase effector domain (GED) in dynamin. The Dnm1p interactions characterized here are similar to those reported for dynamin and dynamin-related proteins that form higher order structures in vivo, suggesting that Dnm1p assembles to form rings or collars that surround mitochondrial tubules. Based on previous findings, a K705A mutation in the Dnm1p GED is predicted to interfere with GTP hydrolysis, stabilize active Dnm1p-GTP, and stimulate a rate-limiting step in fission. Here we show that expression of the Dnm1 K705A protein in yeast enhances mitochondrial fission. Our results provide evidence that the GED region of a dynamin-related protein modulates a rate-limiting step in membrane fission.

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Sec17 (α-SNAP) and an SM-tethering complex regulate the outcome of SNARE zippering in vitro and in vivo

eLife ◽

10.7554/elife.27396 ◽

2017 ◽

Vol 6 ◽

Cited By ~ 16

Author(s):

Matthew L Schwartz ◽

Daniel P Nickerson ◽

Braden T Lobingier ◽

Rachael L Plemel ◽

Mengtong Duan ◽

...

Keyword(s):

Early Stage ◽

Rate Limiting Step ◽

Limiting Step ◽

Trans Complex ◽

Snare Regulators ◽

Rate Limiting

Zippering of SNARE complexes spanning docked membranes is essential for most intracellular fusion events. Here, we explore how SNARE regulators operate on discrete zippering states. The formation of a metastable trans-complex, catalyzed by HOPS and its SM subunit Vps33, is followed by subsequent zippering transitions that increase the probability of fusion. Operating independently of Sec18 (NSF) catalysis, Sec17 (α-SNAP) either inhibits or stimulates SNARE-mediated fusion. If HOPS or Vps33 are absent, Sec17 inhibits fusion at an early stage. Thus, Vps33/HOPS promotes productive SNARE assembly in the presence of otherwise inhibitory Sec17. Once SNAREs are partially zipped, Sec17 promotes fusion in either the presence or absence of HOPS, but with faster kinetics when HOPS is absent, suggesting that ejection of the SM is a rate-limiting step.

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A mutation in the second largest subunit of TFIIIC increases a rate-limiting step in transcription by RNA polymerase III

Molecular and Cellular Biology ◽

10.1128/mcb.14.1.822-830.1994 ◽

1994 ◽

Vol 14 (1) ◽

pp. 822-830

Author(s):

G Rameau ◽

K Puglia ◽

A Crowe ◽

I Sethy ◽

I Willis

Keyword(s):

Rna Polymerase ◽

Rna Polymerase Iii ◽

Structural Motif ◽

Cell Extracts ◽

Rate Limiting Step ◽

Limiting Step ◽

Polymerase Iii ◽

Rate Limiting

In previous studies, we have shown that the PCF1-1 mutation of Saccharomyces cerevisiae suppresses the negative effect of a tRNA gene A block promoter mutation in vivo and increases the transcription of a variety of RNA polymerase III genes in vitro. Here, we report that PCF1 encodes the second largest subunit of transcription factor IIIC (TFIIIC) and that the PCF1-1 mutation causes an amino acid substitution in a novel protein structural motif, a tetratricopeptide repeat, in this subunit. In agreement with the nature of the mutation, in vitro transcription studies with crude extracts indicate that PCF1-1 facilitates the rate-limiting step in transcription, namely, the recruitment of TFIIIB to the template. Additionally, biochemical fractionation of wild-type and mutant cell extracts shows that PCF1-1 increases the amount of the 70-kDa TFIIIB subunit detectable by Western (immunoblot) analysis in purified TFIIIB fractions and the transcription activity of a TFIIIB" fraction containing the 90-kDa subunit of this factor. We suggest that the effect of PCF1-1 on TFIIIB activity in vitro is a consequence of its increased rate of recruitment in vivo.

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A mutation in the second largest subunit of TFIIIC increases a rate-limiting step in transcription by RNA polymerase III.

Molecular and Cellular Biology ◽

10.1128/mcb.14.1.822 ◽

1994 ◽

Vol 14 (1) ◽

pp. 822-830 ◽

Cited By ~ 37

Author(s):

G Rameau ◽

K Puglia ◽

A Crowe ◽

I Sethy ◽

I Willis

Keyword(s):

Rna Polymerase ◽

Rna Polymerase Iii ◽

Structural Motif ◽

Cell Extracts ◽

Rate Limiting Step ◽

Limiting Step ◽

Polymerase Iii ◽

Rate Limiting

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Oxidative regulation of chloroplast enzymes by thioredoxin and thioredoxin-like proteins in Arabidopsis thaliana

Proceedings of the National Academy of Sciences ◽

10.1073/pnas.2114952118 ◽

2021 ◽

Vol 118 (51) ◽

pp. e2114952118

Author(s):

Yuichi Yokochi ◽

Yuka Fukushi ◽

Ken-ichi Wakabayashi ◽

Keisuke Yoshida ◽

Toru Hisabori

Keyword(s):

Redox Regulation ◽

Reducing Power ◽

Photosynthetic Electron Transport ◽

Rubisco Activase ◽

Thermal Dissipation ◽

Fructose 1,6 Bisphosphatase ◽

Related Proteins ◽

Oxidative Regulation

Thioredoxin (Trx) is a protein that mediates the reducing power transfer from the photosynthetic electron transport system to target enzymes in chloroplasts and regulates their activities. Redox regulation governed by Trx is a system that is central to the adaptation of various chloroplast functions to the ever-changing light environment. However, the factors involved in the opposite reaction (i.e., the oxidation of various enzymes) have yet to be revealed. Recently, it has been suggested that Trx and Trx-like proteins could oxidize Trx-targeted proteins in vitro. To elucidate the in vivo function of these proteins as oxidation factors, we generated mutant plant lines deficient in Trx or Trx-like proteins and studied how the proteins are involved in oxidative regulation in chloroplasts. We found that f-type Trx and two types of Trx-like proteins, Trx-like 2 and atypical Cys His-rich Trx (ACHT), seemed to serve as oxidation factors for Trx-targeted proteins, such as fructose-1,6-bisphosphatase, Rubisco activase, and the γ-subunit of ATP synthase. In addition, ACHT was found to be involved in regulating nonphotochemical quenching, which is the mechanism underlying the thermal dissipation of excess light energy. Overall, these results indicate that Trx and Trx-like proteins regulate chloroplast functions in concert by controlling the redox state of various photosynthesis-related proteins in vivo.

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Dynamics of hepatic and peripheral insulin effects suggest common rate-limiting step in vivo

Diabetes ◽

10.2337/diabetes.42.2.296 ◽

1993 ◽

Vol 42 (2) ◽

pp. 296-306 ◽

Cited By ~ 9

Author(s):

D. C. Bradley ◽

R. A. Poulin ◽

R. N. Bergman

Keyword(s):

Rate Limiting Step ◽

Limiting Step ◽

Rate Limiting

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A multi-enzyme cascade for efficient production of d-p-hydroxyphenylglycine from l-tyrosine

Bioresources and Bioprocessing ◽

10.1186/s40643-021-00394-2 ◽

2021 ◽

Vol 8 (1) ◽

Author(s):

Xu Tan ◽

Sheng Zhang ◽

Wei Song ◽

Jia Liu ◽

Cong Gao ◽

...

Keyword(s):

Amino Acids ◽

Specific Activity ◽

Enantiomeric Excess ◽

Efficient Production ◽

Enzyme Cascade ◽

Rate Limiting Step ◽

Limiting Step ◽

Rotation Strategy ◽

Rate Limiting

AbstractIn this study, a four-enzyme cascade pathway was developed and reconstructed in vivo for the production of d-p-hydroxyphenylglycine (D-HPG), a valuable intermediate used to produce β-lactam antibiotics and in fine-chemical synthesis, from l-tyrosine. In this pathway, catalytic conversion of the intermediate 4-hydroxyphenylglyoxalate by meso-diaminopimelate dehydrogenase from Corynebacterium glutamicum (CgDAPDH) was identified as the rate-limiting step, followed by application of a mechanism-guided “conformation rotation” strategy to decrease the hydride-transfer distance d(C6HDAP−C4NNADP) and increase CgDAPDH activity. Introduction of the best variant generated by protein engineering (CgDAPDHBC621/D120S/W144S/I169P with 5.32 ± 0.85 U·mg−1 specific activity) into the designed pathway resulted in a D-HPG titer of 42.69 g/L from 50-g/L l-tyrosine in 24 h, with 92.5% conversion, 71.5% isolated yield, and > 99% enantiomeric excess in a 3-L fermenter. This four-enzyme cascade provides an efficient enzymatic approach for the industrial production of D-HPG from cheap amino acids.

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