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First published online April 22, 2009; 10.1104/pp.109.139170 Plant Physiology 150:606-620 (2009) © 2009 American Society of Plant Biologists OPEN ACCESS ARTICLE
Auxin-Responsive Genes AIR12 Code for a New Family of Plasma Membrane b-Type Cytochromes Specific to Flowering Plants1,[C],[W],[OA]Laboratory of Molecular Plant Physiology, Department of Experimental Evolutionary Biology, University of Bologna, Bologna 40126, Italy (V.P., N.T., P.P., P.T.); Institut de Biochimie et Biophysique Moléculaire et Cellulaire, UMR 8619 (C.M.), and Institut de Biotechnologie des Plantes, UMR 8618 (S.D.L.), CNRS, Université Paris-Sud 11, Orsay F–91405 cedex, France; and Dipartimento di Scienze Chimiche (D.C., M.D.V.) and Dipartimento di Biologia (A.C.), Università di Padova, Padova 35131, Italy
We report here on the identification of the major plasma membrane (PM) ascorbate-reducible b-type cytochrome of bean (Phaseolus vulgaris) and soybean (Glycine max) hypocotyls as orthologs of Arabidopsis (Arabidopsis thaliana) AIR12 (for auxin induced in root cultures). Soybean AIR12, which is glycosylated and glycosylphosphatidylinositol-anchored to the external side of the PM in vivo, was expressed in Pichia pastoris in a recombinant form, lacking the glycosylphosphatidylinositol modification signal and purified from the culture medium. Recombinant AIR12 is a soluble protein predicted to fold into a β-sandwich domain and belonging to the DOMON (for dopamine β-monooxygenase N terminus) domain superfamily. It is shown to be a b-type cytochrome with a symmetrical  -band at 561 nm, fully reduced by ascorbate, and fully oxidized by monodehydroascorbate radical. AIR12 is a high-potential cytochrome b showing a wide bimodal dependence from the redox potential between +80 mV and +300 mV. Optical absorption and electron paramagnetic resonance analysis indicate that AIR12 binds a single, highly axial low-spin heme, likely coordinated by methionine-91 and histidine-76, which are strongly conserved in AIR12 sequences. Phylogenetic analyses reveal that the auxin-responsive genes AIR12 represent a new family of PM b-type cytochromes specific to flowering plants. Circumstantial evidence suggests that AIR12 may interact with other redox partners within the PM to constitute a redox link between cytoplasm and apoplast.
Complex interactions between plant cells and the environment are mediated by the apoplast. The apoplastic liquid phase permeating the cell wall contains relatively low concentrations of solutes (Dietz, 1997  ). Its composition, although largely determined by the protoplast, is easily perturbed by environmental challenges that can thus be perceived by the apoplast and translated into signals that trigger cell responses (Pignocchi and Foyer, 2003; Foyer and Noctor, 2005). Environmental challenges affecting the apoplast commonly result in an oxidative load, caused, for instance, by pollutants (e.g. ozone; Sandermann, 2008) or by endogenously generated reactive oxygen species (ROS). Several enzymatic and nonenzymatic systems are able to generate ROS in the apoplast (Fry, 1998; Apel and Hirt, 2004), an event that is not restricted to biotic or abiotic stresses (Torres and Dangl, 2005), but also involved in diverse physiological conditions, including stomata closure and cell growth (Foreman et al., 2003; Mori and Schroeder, 2004; Gapper and Dolan, 2006; Schopfer and Liszkay, 2006).
Apoplastic reductants not only act as an antioxidant barrier, but they could also modulate oxidative signals, thus actively contributing to plant adaptation to the environment. Ascorbate occurs at 10–4 to 10–3 M concentrations in the apoplast, where it represents the major pool of low-molecular-mass antioxidants (Dietz, 1997
It was suggested (Asard et al., 2001
An ascorbate-reducible cytochrome b from enriched PM preparations was purified as a glycosylated protein of 55 to 63 kD (bean hypocotyls; Trost et al., 2000
In this article, we report on the purification, molecular identification, cloning, and biochemical characterization of the major ascorbate-reducible cytochrome b associated with the PM of soybean (Glycine max) etiolated hypocotyls. The coding gene, known as AIR12 (for auxin induced in root cultures), is early expressed during auxin-induced lateral root formation in Arabidopsis (Laskowski et al., 2006
Purification of PM Ascorbate-Reducible Cytochrome b from Etiolated Soybean Hypocotyls
Purification of PM ascorbate-reducible cytochrome b from etiolated soybean hypocotyls was performed following the protocol described previously for bean hypocotyls (Preger et al., 2005
Protein Identification by Mass Spectrometry Because the soybean genome is not well annotated yet, precautions were taken to avoid false identifications, and two different tandem mass spectrometry (MS/MS) search engines were used. For the 100-kD band, the X!tandem search allowed identification of a soybean EST corresponding to a predicted protein (gene no. Glyma05g04270) as revealed by a BLAST analysis against the soybean genome (http://www.phytozome.net/soybean.php). Using MASCOT, the 100-kD bands were found to correspond to a protein from grape (Vitis vinifera) annotated as a homolog of the multicopper oxidase SKU5 from Arabidopsis (gene no. At4g12420). A multiple sequence alignment with ClustalW (data not shown) revealed that these three candidate proteins share more than 76% identity, indicating that the 100-kD band likely corresponds to a SKU5 multicopper oxidase from soybean. For the band of lower molecular mass (about 60 kD), MASCOT only detected a vegetative storage protein A from soybean (gene no. Glyma07g01730), whereas X!tandem allowed identification not only of this same protein, but also of another protein (gene no. Glyma03g22260) annotated as being similar to Arabidopsis AIR12 (gene no. At3g07390). In addition, peptide mass fingerprints were also performed with the same peptide mixtures as used for nano-liquid chromatography (LC)-MS/MS. For both bands, these analyses confirmed the identifications and increased the sequence coverage. All mass spectrometry (MS) and MS/MS results are summarized in Supplemental Table S1.
The results were further strengthened by the identification of the PM ascorbate-reducible cytochrome b of bean hypocotyls (Preger et al., 2005
AIR12 belongs to the DOMON (for dopamine β-monooxygenase N terminus) domain superfamily, which includes proteins with very different functions, wide phyletic distribution, and different domain architectures (Aravind, 2001
Expression and Purification of Soybean AIR12 in Pichia pastoris
To get better insights into the properties of the AIR12 protein, a modified version of soybean AIR12 cDNA was introduced in the eukaryotic system P. pastoris for heterologous expression. An expression vector pPICZ
RecAIR12 was purified from the culture medium of P. pastoris by means of three chromatographic steps, including a phenyl Sepharose hydrophobic interaction column, followed by an anion-exchange column and gel filtration. The cytochrome eluted from a Superdex 200 gel filtration column as a single symmetric peak of 163 ± 25 kD (n = 6; Fig. 4A
). The ratio A418:A280 of the purified protein attained a value of 2.1. By the pyridine hemochrome method, an extinction coefficient at 418 nm of 113 mM–1 could be determined for recAIR12 hemes under oxidizing conditions. On the other hand, the absorption at 280 nm was contributed both by apoprotein (
Upon deglycosylation of the native purified protein by endoglycosidase H, the apparent molecular mass dropped to 39 kD (Fig. 4B), closer to the theoretical molecular mass of 24 kD of the recombinant protein. The result suggests that the very high apparent molecular mass of the recombinant protein (163 kD) in comparison with the 70 kD of native AIR12, in gel filtration chromatography, may be ascribed to heavy glycosylation by the P. pastoris expression system. In addition, the presence of a 30-amino acid sequence in recAIR12, comprising the C-terminal polyhistidine tag and c-myc epitope, would also contribute to a higher apparent size in gel filtration chromatography (Supplemental Fig. S1). Accordingly, the molecular mass of the glycosylated recombinant protein determined by matrix-assisted laser desorption/ionization time-of-flight (MALDI-TOF) MS analysis was found to be only 37.3 kD. The purified recAIR12 migrates on SDS-PAGE as a high-molecular-mass broad band from 65 to 90 kD, hardly detected by Coomassie staining together with a contaminant of 50 kD (Fig. 5A ). The same high-molecular-mass broad band was intensively stained when the gel was treated for glycoprotein detection (Fig. 5B). After incubation of the purified protein with endoglycosidase H, a strong band of 27 kD appeared in the Coomassie-stained gel, partially overlapping with endoglycosidase H (29 kD), whereas glycoprotein staining failed to reveal any band (Fig. 5). Antibodies directed against AIR12 recognized the diffuse, high-molecular-mass band in nondeglycosylated samples and the band at 27 kD in deglycosylated ones (Fig. 5C). Heme staining of the gel provides qualitative evidence that recAIR12 is a heme binding protein and that heme is noncovalently bound as expected for a b-type cytochrome because most of it is released by recAIR12 and recovered at the bottom of the gel under mild denaturing conditions (lithium dodecyl sulfate [LDS]-PAGE; see "Materials and Methods").
For N-terminal sequencing of recAIR12, purified preparations were blotted on polyvinylidene difluoride (PVDF) membranes after SDS-PAGE and two bands were detected by Coomassie Brilliant Blue staining. Both bands were separately analyzed by Edman degradation and, in each case, two or three amino acids were detected at each cycle. However, both bands gave similar sequences corresponding to two major peptides Gln-Pro-Ala-Val-Ser-Asp-Arg-Tyr-Pro and Val-Ala-Gln-Pro-Ala-Val-Ser-Asp-Arg-Tyr-Pro and another minor peptide Gly-Ile-His-Val-Ala-Gln-Pro-Ala. This suggests that maturation of recAIR12 in P. pastoris generates a small heterogeneity at the N terminus. Nevertheless, all three peptides correspond to the N-terminal sequence of recAIR12, thereby validating the purity of recAIR12 preparations (Supplemental Fig. S1).
Absorption spectra of purified recAIR12 show a symmetric
To check whether recAIR12 could be oxidized by MDA, ascorbate oxidase was added to the reduced cytochrome in the presence of ascorbate (Fig. 8 ). Upon MDA radical generation, a rapid decrease in -band absorption at 561 nm (relative to the isosbestic point at 571 nm) was observed, indicating a rapid oxidation of the cytochrome. The latter could be subsequently rereduced by the addition of higher concentrations of ascorbate.
The EPR spectrum of oxidized recAIR12 shows a ramp-shaped signal with a large gmax value (3.3), and undetectable gmid and gmin (Fig. 9 , trace A). This type of signal, named highly axial low spin (HALS), is commonly exhibited by low-spin hemes when the axial ligands differ from each other and is compatible with Met-91 and His-175 being the heme ligands (Salerno, 1984 ; Zoppellaro et al., 2006). Signals with higher g values are also evident indicating the presence of high-spin ferric heme with both axial (g = 6.0) and rhombic (g = 5.0 and 6.9) components. However, these high-spin components account for only about 3% each of total heme content, suggesting that they originate from partially degraded or misfolded protein. Ascorbate reduction led to complete disappearance of the HALS signal (Fig. 9, trace B), whereas the high-spin components were reduced by dithionite (data not shown). Apart from the g = 4.3 signal due to aspecific iron binding and to the cavity background, no other relevant signals were observed in the EPR spectrum. The signal at about g = 2.0 has not been assigned and may represent one of the components of the high-spin species. Qualitatively similar spectra were observed at both pH 5.5 (Fig. 9) and pH 7.0 (data not shown), further supporting the conclusion that recAIR12 binds a single heme.
Potentiometric redox titrations of recAIR12 at pH 7.0 showed a redox response distributed over more than 200 mV, mostly comprised between +80 and +300 mV (Fig. 10 ). Surprisingly, experimental data could not be properly interpolated by a Nernstian curve for a single redox equilibrium, as expected for a single heme cytochrome. Better interpolations were obtained when two redox equilibria were introduced into the equation (Fig. 10). Two midpoint redox potentials were estimated (Em7 137 ± 19 and 236 ± 21 mV; n = 4), each related to a single redox couple accounting for about one-half of the total redox response (49% ± 16%; n = 4). Redox titrations performed at different pH values (5.5, 7.0, and 7.7) gave almost identical results (data not shown), indicating a very weak pH sensitivity of recAIR12 redox response within physiological pH values.
The capability of plant cells to reduce external electron acceptors by means of a PM redox system is a long-known phenomenon with still scarce molecular basis (Lüthje, 2008 ). In whole cells or intact tissues, reduction of electron acceptors was found associated with apoplast acidification, membrane depolarization, or oxidation of internal electron donors, suggesting a transmembrane electron transfer chain fed by cytosolic reductants (Vuleti et al., 2005). PM vesicles loaded with physiological electron donors [ascorbate, NAD(P)H] were found to reduce impermeable electron acceptors (MDA, ferrichelates, ferricyanide) on the apoplastic side of the membrane (Askerlund and Larsson, 1991; Asard et al., 1992; Horemans et al., 1994; Menckhoff and Lüthje, 2004). In this way, PM redox systems may influence the redox state of the apoplast and provide a redox connection between apoplast and symplast.
Search for molecular components involved in PM redox reactions led to biochemical characterization of several PM redox proteins, including flavoproteins (e.g. quinone reductases; Serrano et al., 1994
Ascorbate-reducible cytochromes with a symmetric
Here, we report that a major ascorbate-reducible cytochrome b of the PM, purified from either soybean or bean etiolated hypocotyls, according to previously published procedures (Preger et al., 2005
Bioinformatic studies predict AIR12 to belong to the DOMON (Aravind, 2001 Purifying adequate amounts of native AIR12 from suitable plant material is a very tedious task, so we have set up a heterologous expression system in P. pastoris. This eukaryotic expression system is also of advantage in that it produces a glycosylated recombinant protein, similar to the native one. The soybean AIR12 gene was transformed in P. pastoris cells into a form with no N-terminal signal peptide and a limited C-terminal deletion to get rid of the GPI anchor. Secreted recAIR12 was purified from culture broth and was found to be glycosylated and soluble in the absence of detergents. The expected molecular mass of the recombinant protein (24 kD) was 13 kD higher due to bound carbohydrates (MALDI-TOF MS). Enzymatic removal of N-glycans gave rise to strongly stained bands at expected positions in SDS gels (Fig. 5).
RecAIR12 shows the typical spectroscopic signature of a cytochrome b with a symmetric
The best fitting of recAIR12 potentiometric redox titrations was obtained when two redox centers were introduced in the Nernst equation. RecAIR12 sensitivity to the redox potential, with two apparent midpoint redox potentials at +137 and +236 mV, is in line with that of partially purified PM cytochrome b from bean hypocotyls (+135 and +204 mV; Trost et al., 2000
The crystallographic structure of DOMON of cellobiose dehydrogenase of the fungus Phanerochaete chrysosporium (Hallberg et al., 2000
The binding of a single heme per molecule is substantiated by different experimental observations, including (1) EPR spectra showing no other low-spin signal than the HALS; (2) the symmetric shape of the
DOMON domains are widespread in nature, usually in association with other redox domains within larger proteins (Ponting, 2001
The role of AIR12 in plant PM redox reactions is still obscure, although an involvement in trans-PM electron transport, and potentially in redox signaling, seems likely. In fact, in ascorbate-loaded PM vesicles, the totality of ascorbate-reducible cytochromes could be oxidized by an external electron acceptor such as ferricyanide or MDA (Asard et al., 1992
A DOMON-plus-cytochrome b561 protein (AC147406_8.1) has recently been detected in lipid rafts of M. truncatula roots together with AIR12 and other redox proteins (Lefebvre et al., 2007
Plant Materials Etiolated seedlings of soybean (Glycine max ‘Pacific’) were grown for 6 d in the dark on moist vermiculite at 25°C.
All chemicals were from Sigma-Aldrich or Merck unless otherwise stated.
Microsomal membranes were prepared as described for bean (Phaseolus vulgaris) hypocotyls (Preger et al., 2005
Chromatographic medium and systems used for purification were from GE Healthcare. Microsomes (35 mg total protein) were solubilized for 1 h at 4°C under stirring, after the addition of 1% (w/v) octyl-β-D-glucopyranoside (OG) and 1 mM ascorbate in 7 mL of solubilization buffer (50 mM Tris-HCl [pH 8.0], 20% glycerol). Detergent-to-protein ratio was 4:1. Insoluble material was sedimented by centrifugation at 110,000g for 30 min at 4°C. Solubilized microsomal proteins (4 mL) were loaded on an anion-exchange SourceQ column (7 mL) equilibrated with 50 mM Tris-HCl (pH 8.0), 20% (v/v) glycerol, 1 mM ascorbate, 1% (w/v) OG. Proteins bound to the resin were eluted with a linear KCl gradient (from 0–0.26 M in 4.7 column volume) at a flow rate of 0.5 mL min–1. Optical absorption of the eluate was continuously monitored at 418 and 427 nm and 0.6-mL fractions were collected. PM cytochrome b-containing fractions, deriving from six anion-exchange separations at pH 8 were pooled together, concentrated to 7 mL (Amicon YM-30 and Centricon YM-30; Millipore), equilibrated with 20 mM 3-(cyclohexylamino)-1-propanesulfonic acid, pH 10.0, 20% (v/v) glycerol, 1 mM ascorbate, 1% (w/v) OG by means of HiTrap fast-desalting cartridges, and reloaded on the anion-exchange SourceQ column equilibrated with the same buffer. A linear KCl gradient (0–0.5 M in 6.3 column volume) was applied at a 0.5 mL min–1 flow rate, and 0.6-mL fractions were collected. Fractions eluted from 0.04 to 0.09 M KCl were pooled together and concentrated to 0.14 mL by Centricon. The cytochrome was finally loaded on a Superdex 200 (HR 10/30) gel filtration chromatography column equilibrated with 50 mM Tris-HCl (pH 8.0), 20% (v/v) glycerol, 1 mM ascorbate, 1% (w/v) OG. Elution was carried out at 0.5 mL min–1 and fractions of 0.2 mL were collected.
HPLC-grade acetonitrile (ACN), Coomassie Brilliant Blue R-250, dithiothreitol, formic acid, iodoacetamide, and trifluoroacetic acid were purchased from Sigma; Tris and Gly from Bio-Rad; and PVDF membrane from Millipore. HPLC-grade ethanol and acetic acid were purchased from VWR.
Bands of interest were excised manually and subjected to in-gel digestion by bovine trypsin (Roche Diagnostics) using the automated protein digestion system DigestPro-96 (Intavis AG). Peptides were extracted first with 1% TFA, then with 60% ACN containing 1% TFA, dried in a SpeedVac concentrator (Savant), and resuspended in 5% ACN/0.1% formic acid. Nano-LC-CHIP-IT-MS/MS experiments were performed on an Agilent 1200 nanoflow LC system coupled to a 6330 ion trap equipped with the Chip Cube orthogonal ionization system (Agilent Technologies). For MS/MS experiments, the system was operated in positive-ion mode with automatic switching between MS and MS/MS modes, whereas MS/MS scanning was performed in the ultrascan resolution mode. A total of six scans were averaged to obtain a MS spectrum, whereas three scans were averaged for the MS/MS spectrum. MS/MS data were analyzed by data analysis software, version 3.4 (Agilent Technologies). Peptide mass fingerprints were also performed by MALDI-TOF MS as described previously (Marchand et al., 2006 For automated Edman degradation, peptides from in-gel tryptic digest of a purified sample were first subjected to HPLC separation on a C-18 reverse-phase column. Automated Edman degradation of two peptides was performed with an Applied Biosystems Procise 494 cLC protein sequencer at the W.M. Keck Facility.
Heme content of recAIR12 samples was analyzed using the pyridine hemochrome method as described in Metzger et al. (1997)
Total protein was assayed by the method of Bradford. RecAIR12 content was calculated from dithionite-reduced minus oxidized spectra (
An EST clone containing the full-length soybean AIR12 cDNA (GenBank accession no. FJ528079) was purchased from Biogenetic Services and used as a template for PCR. Two oligonucleotide primers were designed for ligation of a truncated form of AIR12 cDNA into the KpnI site of the expression vector pPICZ
Chromatographic medium and systems used for purification were from GE Healthcare. Two days after induction, cultures of P. pastoris X-33/pPICZ
For protein deglycosylation Endo H (New England BioLabs) was used according to the manufacturer's instructions. Incubation of denatured samples with Endo H was carried out at 37°C for 1 h. For deglycosylation of the native nondenatured protein, the incubation was done overnight at 22°C.
A truncated form of soybean AIR12 lacking the N-terminal signal peptide and C-terminal hydrophobic signal peptide (see Fig. 3) was cloned into the expression vector pET-28a(+) (Novagen) and expressed into Escherichia coli BL-21(DE3) cells according to Sparla et al. (1999)
SDS-PAGE was performed on 12.5% acrylamide gels. Samples were boiled for 10 min in sample buffer prior to loading. Gels were stained with Coomassie Brilliant Blue R-250. The staining of glycoproteins was done according to Leach et al. (1980)
To visualize hemoproteins, recAIR12-containing samples were resolved on 12.5% PAGE, using LDS in the gel, sample, and running buffer instead of SDS, according to the method of Sinclair et al. (1981) For western blotting, proteins were separated by SDS-PAGE and electroblotted (semidry cell; Schleicher-Schuell) onto nitrocellulose membranes. Membranes were stained with Red Ponceau before incubation with rabbit antiserum raised against AIR12 expressed in E. coli (see above), and peroxidase-conjugated secondary antibodies. Primary and secondary antibodies were diluted 1:2,000 and 1:1,000, respectively. Blots were developed by chemiluminescence according to standard procedures.
After deglycosylation treatment with EndoH, proteins were separated by 12% SDS-PAGE and electroblotted onto PVDF membranes (pore size 0.2 µm) using the liquid Mini Trans-Blot Cell (Bio-Rad). Bands detected by Coomassie Brilliant Blue R-250 staining were cut and subjected to automated Edman degradation using a Procise sequencer (Applied Biosystems).
The molecular weight of recAIR12 was determined by MALDI-TOF MS without the desalting step, as described previously (Zaffagnini et al., 2007
Spectrophotometric titrations were performed essentially as described in Venturoli and Zannoni (1988)
Samples containing 120 µM purified recAIR12 dissolved in 50 mM MES-KOH, pH 5.5, 150 mM KCl were withdrawn into EPR tubes. Oxygen was removed by flushing nitrogen above the solutions in the EPR tubes. The samples were flash cooled in liquid nitrogen before insertion in the EPR spectrometer at 10K. Continuous-wave EPR measurements were performed on a Bruker Elexsys E580 spectrometer at 9.4 GHz, equipped with standard TE102 cavity. The temperature was controlled with a helium flow cryostat (Oxford Instruments ESR-900) driven by a temperature controller. Reduction of the samples was obtained by adding a few microliters of a concentrated ascorbate solution (final concentration approximately 5 mM) directly in the EPR tubes. Further reduction was achieved by adding sodium dithionite (few grains). Experimental conditions were T = 10K, microwave power = 2 mW, field modulation = 100 kHz, modulation amplitude = 10 G, time constant = 82 ms, conversion time = 164 ms; g values were estimated by calibration with a diphenylpicrylhydrazyl sample. Spin quantification of the high-spin hemes relative to the HALS species was performed by simulation of the X-band EPR spectrum and double integration of the contribution of each individual species.
All proteins containing a DOMON domain (IPR005018) from Arabidopsis (Arabidopsis thaliana) and rice (Oryza sativa ‘japonica’ group) were identified in the INTERPRO database (http://www.ebi.ac.uk/interpro). AIR12 sequences were identified by BLASTp searches in the National Center for Biotechnology Information (NCBI) protein database (http://www.ncbi.nlm.nih.gov) and in sequenced genomes in Joint Genome Institute databases (http://genome.jgi-psf.org). Additional sequences were retrieved by tBLASTn searches in NCBI GenBank and dbEST databases. For each EST identified, the corresponding Unigene cluster was retrieved (http://www.ncbi.nlm.nih.gov/unigene) and used for EST assembly with the CAP3 program (Huang and Madan, 1999 Sequence data from this article can be found in the GenBank/EMBL data libraries under accession numbers FJ528079 and FJ535652.
The following materials are available in the online version of this article.
Received March 31, 2009; accepted April 15, 2009; published April 22, 2009.
1 This work was supported by the Ministero della Pubblica Istruzione (grants FIRB 2004 and PRIN 2007). 
2 These authors contributed equally to the article. The author responsible for the distribution of materials integral to the findings presented in this article in accordance with the policy described in the Instructions for Authors (www.plantphysiol.org) is: Valeria Preger (valeria.preger{at}unibo.it).
[C] Some figures in this article are displayed in color online but in black and white in the print edition.
[W] The online version of this article contains Web-only data.
[OA] Open access articles can be viewed online without a subscription. www.plantphysiol.org/cgi/doi/10.1104/pp.109.139170 * Corresponding author; e-mail valeria.preger{at}unibo.it.
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ABSTRACT
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561–571) of 21 mM–1, as determined by the pyridine hemochrome method with the assumption that AIR12 binds a single heme (see below). The absorption maximum of the pyridine hemochrome at 557 nm strongly suggested that recAIR12 binds indeed a b-type heme (Porra and Jones, 1963
-band at 427 nm (
-aminolevulinic acid and 40 µM hemin. Cultures were grown (28°C, 220 rpm) for 48 h in inducing medium with the addition of 1% (v/v) methanol every 24 h.