Exploring Regulation Genes Involved in the Expression of L-Amino Acid Oxidase in Pseudoalteromonas sp. Rf-1

Bacterial L-amino acid oxidase (LAAO) is believed to play important biological and ecological roles in marine niches, thus attracting increasing attention to understand the regulation mechanisms underlying its production. In this study, we investigated genes involved in LAAO production in marine bacterium Pseudoalteromonas sp. Rf-1 using transposon mutagenesis. Of more than 4,000 mutants screened, 15 mutants showed significant changes in LAAO activity. Desired transposon insertion was confirmed in 12 mutants, in which disrupted genes and corresponding functionswere identified. Analysis of LAAO activity and lao gene expression revealed that GntR family transcriptional regulator, methylase, non-ribosomal peptide synthetase, TonB-dependent heme-receptor family, Na+/H+ antiporter and related arsenite permease, N-acetyltransferase GCN5, Ketol-acid reductoisomerase and SAM-dependent methytransferase, and their coding genes may be involved in either upregulation or downregulation pathway at transcriptional, posttranscriptional, translational and/or posttranslational level. The nhaD and sdmT genes were separately complemented into the corresponding mutants with abolished LAAO-activity. The complementation of either gene can restore LAAO activity and lao gene expression, demonstrating their regulatory role in LAAO biosynthesis. This study provides, for the first time, insights into the molecular mechanisms regulating LAAO production in Pseudoalteromonas sp. Rf-1, which is important to better understand biological and ecological roles of LAAO.


Introduction
L-Amino acid oxidase (LAAO; EC 1.4.3.2) is usually a flavin adenine dinucleotide (FAD)containing homodimeric protein, which functions in stereospecific oxidative deamination of L-amino acids to the corresponding a-keto acids with release of NH 4 + and H 2 O 2 [1]. It plays important biological roles, such as apoptosis [2], cytotoxicity [3], edema [4], hemolysis, hemorrhage [5], inducing or inhibiting platelet aggregation [6], and parasite-killing and antimicrobial activities [7]. Most of its biological functions are associated with the produced H 2 O 2 which is toxic to most organisms [8,9]. Therefore, LAAO is considered as a toxic protein and characterization of the mechanisms controlling its expression is very important for understanding not only its biological but also ecological roles. The enzymatic and physiochemical properties, biological function and structure of LAAO as well as its cloning and heterologous expression have been intensively investigated [9]. However, studies on unraveling the mechanism regulating LAAO expression are limited, where only a few genes controlling its transcription and translation have been explored. Previously, it was found that LAAO activity in Neurospora crassa can be induced by L-Phe, D-Phe, ATP and cycloheximide. Those inducing agents can regulate the lao gene expression at transcriptional level [10]. However, the regulation genes were undefined. More recently, a spontaneous mutant of N. crassa gln-1br8 with deficiency in glutamine synthetase β polypeptide was confirmed to have higher LAAO activity [11]. Again, the relevant genes for regulation were unexplored. It was also reported that LAAO activity in N. crassa can be induced through addition of L-amino acids to nitrogen-starved cultures as well as addition of protein synthesis inhibitors or Damino acids [12,13]. LAAO expression was regulated by NIT2 and the nmr gene product at transcriptional level [14]. Besides LAAO in N. crassa, LAAO from Marinomonas mediterranea was found to be regulated by hybrid sensor histidine kinase PpoS at transcriptional level [15]. Two genes of lodAB operon were found to be necessary for LAAO expression in M. mediterranea [16].
LAAO is widely found in marine Pseudoalteromonas spp. [17][18][19] and plays an important role in dispersal and colonization across a range of Gram-negative marine bacteria, such as Pseudoalteromonas tunicate [20], suggesting its important ecological function in marine environment. Recently, a yellow-pigmented marine bacterium Pseudoalteromonas sp. B-3 was isolated to produce LAAO [21,22]. In this study, to explore the genes involved in regulating LAAO activity, a red-pigmented spontaneous mutant strain of Pseudoalteromonas sp. B-3 resistant to rifampicin, designated as Pseudoalteromonas sp. Rf-1, was selected. The transposon mutagenesis [23] was used to construct a mutant library of strain Rf-1 and the target mutants with altered LAAO activity were screened using Prussian blue agar assay method [22]. Based on genetic and enzymatic analysis, several regulation genes were identified. Our results shed some lights into the molecular mechanisms regulating LAAO activity in this marine bacterium across the natural environment.

Mutant screening of LAAO activity
To explore the genes regulating LAAO activity in Pseudoalteromonas sp. Rf-1, plasmid pLOF/Km carrying a mini-Tn10 [24] was used to generate a mutant library of strain Rf-1. Antibiotics of rifampicin (Rif) and kanamycin (Km) were used to repress Escherichia coli with plasmid pLOF/Km and wild type strain Rf-1, respectively. After transposon mutagenesis [23,25], approximately 4,000 mutants appeared on marine medium (MM) plate with Rif and Km. Then, culture supernatant of individual mutant was subjected to LAAO-activity screening with Prussian blue agar assay [22]. Altered LAAO activity was detected in 300 mutants,(data not shown) in which 15 mutants displayed significant altered or abolished LAAO activity (Fig. 1). As shown in Table 1, compared to wild-type strain, 3 mutants (B3, B21 and B22) gave increased LAAO activity, 8 mutants (B9, A15, A45, B20, B17, A60, B10 and B11) yielded decreased LAAO activities, while the other 4 mutants (B19, B12, B6 and B1) showed null LAAO activity. The statistical analysis showed that the mean difference of blue halo diameter or LAAO activity between mutant and wild type was all extremely significant (P<0.001) ( Table 1). Therefore, these 15 mutants were selected for further investigation. Measurement of LAAO activity from the LAAO-altered or -deficient mutants using Prussian blue agar assay [22]. 50 μl of culture supernatant of individual mutant or wild-type strain Rf-1 was added into the punched circular hole with a diameter of 6 mm in the Prussian blue agar assay plate for color development from Berlin green to blue caused by H 2 O 2 produced by LAAO activity. The diameter of the resultant blue halo is exponentially associated with the LAAO activity. Compared with wild-type strain, the mutants B3, B21 and B22 had the increased LAAO activities, and the mutants B9, A15, A45, B20, B17, A60, B10 and B11 yielded the decreased LAAO activities, while the mutants B19, B12, B6 and B1 were deficient in LAAO activity.

Molecular confirmation of transposon insertion in mutants
Two primer pairs were used to confirm the correct insertion of mini-Tn10 gene along with Km resistance marker gene (IS-km-IS) in the 15 mutants from above. One pair was Tn10KAP3 (5'-CATTTGATGCTCGATGAGTTTTTCT-3') and S1 (5'-TTGGTAAAAATCATTAAGT-TAAGGT-3'), which were both specific to IS-km-IS region; the other pair was DTn10AP3 (5'-CGTTGCGCTGCCCGGATTACAGCCG-3') and Q2 (5'-AAACGATGCCCATTTTGTT-GATTAT-3'), which were specific to IS-km-IS and pLOF vector region (outside of IS-km-IS), respectively. The first primer pair was used to amplify a 506bp fragment, while the second one was use to amplify a 964bp fragment. As shown in Fig. 2, positive control of pLOF/Km yielded both fragments, while negative control (wild type strain Rf-1) gave neither. Mutants A60 and A15 exhibited neither fragment, suggesting unclear mutation or failure of PCR amplification; mutant A45 unexpectedly displayed both fragments, probably due to insertion of extra piece from pLOF/Km vector or even whole pLOF/Km. On the other hand, all the remaining 12 mutants expectedly gave only one fragment (506 bp) from primer pair of Tn10KAP3 and S1, but not the other one (964 bp) from primer pair of DTn10AP3 and Q2. All these results indicated that the correct insertion of IS-km-IS took place probably only in 12 mutants (B3, B21, B22, B9, B10, B11, B17, B20, B1, B6, B12 and B19) which were used in the following experiments. PCR detection of insertion of mini-Tn10 together with kanamycin resistance marker (IS-km-IS region) in LAAO-altered mutants. S: PCR using primers Tn10KAP3 and S1; Q: PCR using primers DTn10AP3 and Q2; pLOF: PCR using plasmid pLOF/Km as template (positive control); Rf-1: PCR using genomic DNA of wild type strain Rf-1 as template (negative control); B3, B21, B1, B12, B19, A45, B6, B9, B10, B11, B20, A60 and A15: PCR reaction using genomic DNA from the corresponding mutant as template. Quantitative real-time PCR (qRT-PCR) analysis of the differential expression of lao gene The expression of lao gene in 12 mutants identified above and wild-type strain was measured by qRT-PCR [26]. The results in Fig. 3 showed that all the strains yielded the expression of lao gene. Compared to wild-type strain Rf-1, 3 mutants (B3, B21, and B22) had increased expression of lao gene, while the other 9 gave decreased expression. Overall, the qRT-PCR results showed the same tendency as LAAO enzymatic activity in the different mutants. In mutants with null activity, the qRT-PCR gave also lower levels of mRNA, while in mutants with higher LAAO activity it is possible to see higher mRNA levels ( Fig. 1 and Table 1). Notably, the mutants (B1, B6, B12 and B19) with abolished LAAO activity still exhibited lao gene expression. Statistical analysis indicated that the mean difference of relative lao gene expression between mutant and wild type was significant (P<0.05) in mutants B19 and B17, and extremely significant (P<0.001) in mutants B1, B6, B12, B9, B10, B11, B20, B3 and B21, but not significant (P>0.05) in mutant B22. However, regarding LAAO activity, the mean differences between mutants and wild type all were extremely significant (P<0.001). Thus, all these findings indicated that LAAO activity and the corresponding lao gene expression are probably regulated by the disrupted genes in different mutants at different levels.

Characterization of the genes disrupted by transposon in mutants
The DNA region flanking inserted transposon was sequenced for identification of the disrupted gene in each mutant. Typically, a DNA sequence with around 500-1200 bp for each mutant was obtained through hiTAIL-PCR [27]. As shown in Table 2, most of the sequences in mutants could match with the genes from the same genus, Pseudoalteromonas rubra ATCC 29570, with the exception that mutant B10 showed the highest similarity (68%) to a gene coding for TonB-dependent heme receptor family in Alcanivorax dieselolei B5. The disrupted gene resulting in increase of LAAO activity in mutant B22 showed the highest identity (72%) to a gene encoding GntR family transcriptional regulator. The possible corresponding genes resulting in decrease of LAAO activity in mutants B20, B17 and B10 had the closest similarity to the genes coding for methylase (80%), non-ribosomal peptide synthetase (82%) and TonBdependent heme receptor family (68%), respectively. Interestingly, the disrupted genes in mutants B1, B6, B12 and B19 with abolished LAAO activity had the highest similarity to those coding for SAM-dependent methytransferase (80%), Ketol-acid reductoisomerase (80%), Nacetyltransferase GCN5 (80%), and Na + /H + antiporter NhaD and related arsenite permease (81%), respectively. Besides, the disrupted genes in mutants B3 and B9 yielded no any similar gene in databases and the ones in mutants B21 and B11 all matched with the unannotated sequences. Therefore, we did not try to propose the function of these 4 genes. All the characterized gene sequences have been deposited in GenBank and the corresponding access no. was included in Table 2.

Complementation of the disrupted genes in mutants with abolished LAAO-activity
The transposon-disrupted genes in the 4 mutants with null LAAO-activity (B1, B6, B12 and B19) were identified as sdmT, karI, nat5 and, nhaD with their corresponding functions displayed in Table 2. To further confirm that these identified genes were involved in regulation of LAAO biosynthesis, we tried to perform gene complementation in each mutant. We retrieved the full gene sequences of sdmT (access no. KP191657), karI (access no. KP191658) and nhaD (access no. KP191659), with length of 594 bp, 1473 bp and 1455 bp, respectively. However, the retrieval of full nat5 gene failed, even after extensive optimization procedure on hiTAIL-PCR condition. Subsequently, the 3 successfully retrieved genes were cloned into vector pBBR1MCS-5 [28] to form pBBR1MCS-5/sdmT, pBBR1MCS-5/nhaD and pBBR1MCS-5/karI, respectively. The pBBR1MCS-5/sdmT and pBBR1MCS-5/nhaD were successfully transformed into mutants B1 and B19, respectively, with assistance of plasmid pBR2013 [29] in E. coli DH5α. However, the transformation of pBBR1MCS-5/karI into mutant B6 failed. Prussian blue agar assay in Fig. 4 showed that the two complemented strains (complons), B1/MS and B19/MN yielded the Prussian blue halos with comparable diameter to wild-type strain Rf-1, indicating that LAAO activity was nearly completely recovered. Accordingly, our data demonstrated that both sdmT gene and nhaD gene are involved in controlling LAAO biosynthesis in Pseudoalteromonas sp. Rf-1. As shown in Fig. 5, the relative expression level of lao gene in either mutant B1 or mutant B19 was extremely significantly (P<0.001) decreased, compared to that in wild-type Rf-1. The complons B1/MS and B19/MN resulted from the complementation of sdmT gene and nhaD gene in B1 and B19, respectively, exhibited extremely significant (P<0.001) increase of lao gene expression, as compared to original mutants. In addition, their lao gene expression levels were comparable to that in wild-type Rf-1 (no significance, P>0.05), suggesting that the complementation of transposon-inserted genes can almost completely restore lao gene expression. The negative control using complons B1/M and B19/M with blank complementation lack of gene of interest displayed similar expression level as original mutants (no significance, P>0.05). Taken together, we concluded that both sdmT gene and nhaD gene upregulate the lao gene expression at transcriptional level in Pseudoalteromonas sp. Rf-1. Moreover, considering that the disruption of sdmT gene and nhaD gene resulted in completely undetectable LAAO activity, but only partial decrease of lao gene expression, we proposed that both genes also regulated LAAO biosynthesis probably at posttranscriptional level in Pseudoalteromonas sp. Rf-1.

Discussion
Species of the genus Pseudoalteromonas, in particular color-pigmented ones, are generally found to be associated with marine eukaryotes and have antibacterial, algicidal, antifungal, or antiviral activity. Several Pseudoalteromonas isolates specifically deter the settlement of common marine fouling organisms. Thus, Pseudoalteromonas cells are advantageous in their contest for nutrients, space and colonization of surfaces, and are protected against predators grazing at surfaces [30,31]. LAAO is believed to be associated with Pseudoalteromonas' biological and ecological roles in marine environment [30,31]. Therefore, a thorough understanding of mechanisms controlling LAAO production is extremely important and is attracting a great number of interests.
Despite the prevalent application of mutagenesis technique, such as transposon mutagenesis, in mutant screening since the past decade, applying the detection method cheaply and efficiently for large-scale screening of mutants with different LAAO activities has proven challenging [32]. To date, very little is known about the regulation mechanism underlying LAAO transcription and production in marine bacteria. Previously, Prussian blue agar assay method has been developed with high efficiency and convenience, holding a promising application as a sensitive procedure for differentiating the mutants from a mutant library with altered LAAO activity [22]. In this study, over 4,000 mutants with Rif and Km resistance were isolated and screened using Prussian blue agar assay, where only about 300 (7.5%) mutants in total were found to have altered LAAO activity. Among them, more than 95% mutants only had slight changes in LAAO activity, resulting in the difficulty for clear differentiation of mutants, which in the future could be overcome by using ferric-xylenol orange formation (Fe Ⅲ -XO) agar assay method with higher sensitivity [32,33] for detecting LAAO activity. Nevertheless, the combination of mini-Tn10 mutagenesis with Prussian blue agar assay allowed us to successfully identify several genes potentially controlling LAAO production in Pseudoalteromonas sp. Rf-1. Those identified genes could be grouped into two categories, positive regulator and negative regulator, based on the change of LAAO activity in mutants listed in Table 2.
The only identified negative regulator is GntR family transcriptional regulator that was found in mutant B22. The GntR family is one of the most abundant and widely distributed groups of transcriptional regulators in bacteria [34]. It was reported that the gntR gene acts to repress transcription of itself as well as a series of genes immediately adjacent to it [35,36]. Mutation of gntR gene resulted in increased LAAO activity, indicating a downregulation role of gntR gene in Pseudoalteromonas sp. Rf-1 for LAAO biosynthesis. In addition, our data showed that its disruption only caused slight increase of lao gene expression. This could suggest that the gntR gene probably downregulates some genes at transcriptional level which in turn regulate LAAO production at posttranscriptional level. However, this postulation remains to be further determined.
On the other hand, we identified 7 possible genes that are likely involved in upregulation pathway of LAAO activity. Three of proposed genes coding for TonB-dependent heme receptor family protein (TdhR), non-ribosomal peptide synthetase (NrpS) and methylase led to decreased LAAO activity after mutation. TdhR is predicted to localize at bacterial membrane, and can sense signals from extracellular or intracellular messengers and transfer them across membrane, leading to transcriptional activation of target genes [37]. The disruption of this gene resulted in extremely significant (P<0.001) decrease of lao gene expression, thus suggesting that the tdhR gene in Pseudoalteromonas sp. Rf-1 may positively regulate LAAO biosynthesis at transcriptional level. Moreover, TdhR protein can interact with outer membrane receptor that can carry specific substrates into cytoplasm space [37]. Thus, it is possible that TdhR may also be involved in absorption of substrates for LAAO biosynthesis. The NrpS protein is generally responsible for introduction of amino acid, and can control the production level of the corresponding peptides. Besides, NrpS also has formyltransferase activity and hydroxymethytransferase activity. Therefore, the NrpS protein may affect the substrate absorption for LAAO biosynthesis and posttranscriptional modification of LAAO. Moreover, our data indicated that the disruption of nrpS gene extremely significantly (P<0.001) decreased lao gene expression, suggesting that nrpS gene in Pseudoalteromonas sp. Rf-1 probably participates in upregulation of LAAO biosynthesis at transcriptional level, too. Similarly, considering that the insertion of transposon into methylase gene in mutant B20 resulted in both extremely significant (P<0.001) decrease of lao gene expression and extremely significant (P<0.001) decrease of LAAO activity, we postulated that this gene is potentially involved in upregulation of LAAO biosynthesis at transcriptional level.
Finally, we identified 4 upregulating genes that would abolish LAAO activity if disrupted. The disrupted gene in mutant B19 probably codes for Na + /H + antiporter NhaD and related arsenite permease (NhaD). NhaD is a ubiquitous protein usually in cytoplasmic membrane and in membranes of many organelles, and plays a primary role in homeostatic mechanisms and transmembrane transport of substances, such as H 2 O 2 , protein and vitamins. It is proposed that the disruption of this gene may disturb LAAO secretion. In addition, the disruption of this gene caused significant decrease (P<0.05) of lao gene expression, thus suggesting that the nhaD gene in Pseudoalteromonas sp. Rf-1 may also indirectly upregulate LAAO biosynthesis at transcriptional level. The disrupted genes in mutants B12 and B1 matched with the ones encoding N-acetyltransferase GCN5 (NaT5) and SAM-dependent methytransferase (SdmT), respectively. These two proteins are responsible for acetylation of Lys and Cys residues, and methylation of Glu, His, Lys and Arg residues, respectively, both participating in posttranslational modification of proteins [38]. These amino acid residues account for a huge amount of amino acids in LAAO of Pseudoalteromonas sp. Rf-1 (data not shown). Thus, NaT5 and SdmT may play a role in posttranslational modification of LAAO. Besides, NaT5 is responsible for acetylating the wobble base of elongator tRNA Met by utilizing acetyl-coenzyme A (CoA) and ATP (or GTP) to form N 4 -acetylcytidine (ac4C) [39]. The ac4C formation at wobble base of elongator tRNA Met is thought to ensure the precise recognition of AUG codon by preventing misreading of near-cognate AUA codon [39,40], thus ensuring the correct initiation of protein translation of protein. SdmT can catalyze 2'-O-methylation of cytidine 1402 and N 4 -methylation of cytidine 1402 in 16S rRNA. It has been found that methylation modification in 16S rRNA is necessary for stringent selection of the initiator tRNA and efficient translation initiation at UUG and GUG [41,42]. All these suggest that both nat5 and sdmT genes in Pseudoalteromonas sp. Rf-1 may positively regulate the translation initiation of LAAO as well. Considering the fact that the disruption of these two genes extremely significantly (P<0.001) downregulated lao gene expression, it is clear that both genes are probably involved in positive regulation on LAAO biosynthesis also at transcriptional level. The disrupted gene in another mutant B6 with no LAAO-activity matched with the one coding for ketol-acid reductoisomerase (KarI). This enzyme can catalyze conversion of acetohydroxy acids into dihydroxy valerates, which is a synthetic pathway of the essential branched side chain of amine acids Val and Ile. Probably, the disruption of karI gene in Pseudoalteromonas sp. Rf-1 will affect the synthesis of amino acids Val and Ile in LAAO, thus leading to loss of LAAO activity. Since the karI gene disruption extremely significantly (P<0.001) downregulated lao gene expression, it is clear that the karI gene positively regulates LAAO biosynthesis also at transcriptional level.
To our best knowledge, it is the first time to explore many genes involved in regulation of LAAO activity in Pseudoalteromonas sp. Rf-1 at transcriptional, posttranscriptional, translational and/or posttranslational level. Although western blot and/or site-directed mutation will be desired to confirm the molecular function of the explored genes in LAAO biosynthesis, our findings pave a road for exploiting the mechanisms underlying LAAO biosynthesis and secretion, and provide the understanding of biological and ecological roles in Pseudoalteromonas sp. Rf-1 by controlling LAAO activity in marine environment.

Strains, plasmids and media
All bacterial strains and plasmids used in this study were shown in Table 3. Pseudoalteromonas sp. Rf-1 (Rif r ) was grown in a marine medium (MM) (0.3% yeast extract, 0.5% peptone, 3% sea salt (Sigma)) at 28°C with a shaking of 120 rpm. All E. coli cells were cultured in Luria-Bertani (LB) medium at 37°C with a shaking of 150 rpm. Unless otherwise specified, to make solid medium, agar was added to a final concentration of 2%. When required, antibiotics were added to medium with final concentrations as below: rifampicin (Rif) 50 μg/ml, ampicillin (Ap) 100 μg/ml, gentamicin (Gm) 50 μg/ml, streptromycin (Str) 50 μg/ml and kanamycin (Km) 50 μg/ml.

Conjugation and transposon mutagenesis
To generate mutants with altered LAAO activity, transposon mutagenesis [23,25] was performed in rifampicin-resistant Pseudoalteromonas sp. Rf-1. In brief, the strain Rf-1 was inoculated into MM with 50 μg/ml Rif and the E. coli S17-1(λpir) harboring suicide vector pLOF/Km inoculated into LB (0.5% NaCl) with 100 μg/ml Ap and 50 μg/ml Km. After overnight incubation, both strains were reinoculated into their own fresh medium without antibiotics and allowed to reach exponential growth phase. To transfer the mini-Tn10 transposon together with kanamycin resistance marker on pLOF/Km to strain Rf-1 cells through conjugation, a 40 μl sample of the exponentially growing recipient Rf-1 cells was spotted onto the surface of conjugation medium (LB-MM, obtained by mixing equal amounts of the two media) agar plate and allowed to dry before another 40 μl of E. coli donor cells were added to the top of previous spot. Controls with only strain Rf-1 or E. coli were also prepared. After overnight conjugation, the cells were then collected by scraping and suspended in 1 ml of MM. After appropriate dilution, the cells were plated onto selective MM with 50 μg/ml Rif and 50 μg/ml Km, and incubated at 28°C for 48 h. Finally, the target mutants with altered LAAO activity were screened using Prussian blue agar assay method [22].

Prussian blue agar assay for screening of mutants with altered LAAO activity
Mutants with deficient or altered LAAO activity were selected based on high throughput ingel determination method of Prussian blue agar assay [22]. In brief, individual mutant was grown in MM with Rif and Km for 2 d at 28°C with a shaking of 160 rpm. After measurement of absorbance reading (600 nm) and adjustment of cell density if necessary, 1 ml of the above culture was added to 250 ml conical flask containing 50 ml of MM with Rif and Km for fermentation at 28°C with shaking at 160 rpm. After 72-h fermentation, the culture supernatant was harvested with a centrifugation at 5 000 rcf (relative centrifugal force) for 10 min at 4°C. Then, the Prussian blue agar assay plate containing 1.0 g/l FeCl 3 Á6H 2 O, 1.0 g/l potassium Table 3. Bacterial strains and plasmids used in this study.

Determination of transposon-inserted gene
Genomic DNAs were extracted from the transposon-inserted mutants of strain Rf-1 using a bacterial genomic DNA extraction kit (GE, USA). The DNA sequence flanking the inserted transposon in a mutant was determined using high-efficiency thermal asymmetric interlaced PCR (hiTAIL-PCR) [27] (first time). The primers used for hiTAIL-PCR were shown in Table 4. In the first round, PCR was performed in 20 μl of reaction mixture containing 2.0 μl of PCR buffer, 200 μM dNTPs, 1.0 μM of any one of the LAD primers [27], 50 nM DTn10AP1, Table 4. Primers used in high-efficiency thermal asymmetric interlaced PCR.  Table 5. The PCR products from the second or third round of PCR amplification were electrophoresed on a 1.5% agarose gel and the desired amplicons were purified using a gel extraction kit (Qiagen, CA, USA) for TA cloning with pMD19-T simple vector (TaKaRa, Dalian, China). After sequencing by Sangon Biotech (Shanghai, China), the intermediate sequences of disrupted genes in mutants were collected and compared with the relevant genes in the GenBank of NCBI, EMBI databases and/or Prosite. To retrieve the entire length of sdmT, karI and nhaD gene sequences from LAAO-deficient mutants B1, B6 and B19, respectively, the hiTAIL-PCR was employed again (second time) to amplify the 5'-and 3'-regions of sdmT, karI and nhaD genes. As shown in Table 2, specific primer sets were designed based on the intermediate region collected from the first time of hiTAIL-PCR. After hiTAIL-PCR (Table 3), the desired products were recovered from agarose with gel extraction kit for TA cloning. After sequencing, the contigs of 5'-region, intermediate region, and 3'-region were assembled for analysis.

Complementation of the disrupted genes through tri-parental mating
To complement the disrupted genes of sdmT, karI and nhaD in three mutants of B1, B6 and B19, respectively, the entire three genes of sdmT, karI and nhaD were individually amplified using three primer pairs (Table 6), SdmtF and SdmtR, KariF and KariR, and NhaDF and NhaDR, respectively. The Pfu DNA polymerase (Promega, USA) was used to amplify 594 bp of sdmT gene, 1473 bp of karI gene and 1455 bp of nhaD gene. After addition of 3'-adenine overhang by Taq DNA polymerase (TaKaRa, Dalian, China), the desired PCR product was gel- The Genes Regulating LAAO Expression in Pseudoalteromonas sp. Rf-1 purified and cloned into pMD19-T simple vector. After digestion with Hind III/EcoR I, Kpn I/ Hind III and Kpn I/Xba I, the sdmT-gene, karI-gene and nhaD-gene fragments were individually cloned into expression vector pBBR1MCS-5 [28] to yield recombinant plasmids pBBR1MCS-5/sdmT, pBBR1MCS-5/karI and pBBR1MCS-5/nhaD, respectively, and separately transformed into E. coli HB101. Then, with assistance of plasmid pBR2013 [29] in E. coli DH5α, these three constructed plasmids were introduced into mutants B1, B6 and B19, respectively, for complementation of the corresponding disrupted gene into each mutant cell through tri-parental conjugation which was performed as below. First, the mutant of strain Rf-1 (receptor), E. coli HB101 with corresponding recombinant plasmid (donor) and E. coli DH5α with pBR2013 (assistor) were separately inoculated into MM with 50 μg/ml Rif and 50 μg/mL Km, LB with 50 μg/ml Gm and LB with 50 μg/ml Km, respectively, and allowed to reach exponential growth phase. Then, 2 ml of each culture was centrifugated at 2 000 rcf for 5 min to collect the cells. After washing once, each cell pellet was resuspended in 0.5 ml of conjugation medium (mixture of 1/2 MM and 1/2 LB) and three resuspensions were mixed together for another centrifugation at 5 000 rcf for 5 min. After removal of supernatant, the cell mixture of mutant, HB101 and DH5α was resuspended in 0.2 ml of conjugation medium and dropped to sterilized microporous membrane (size diameter 1 cm; aperture 0.45 μm) on conjugation medium plate for overnight conjugation at 30°C. Finally, the microporous membrane was transferred to 3 ml of MM for washing with vortex. After appropriate dilution, 50 μl of cell solution was spread on MM with 50 μg/ml Rif, 50 μg/ml Km and 50 μg/ml Gm. After incubation at 30°C, the target colonies were confirmed with molecular analysis and used for detection of LAAO activity and lao gene expression.

Analysis of lao gene expression by qRT-PCR
To measure the lao gene (access no. KP165133 in GenBank) expression, qRT-PCR [26] was used to amplify cDNA products reversely transcribed from mRNA of mutants selected. In brief, individual mutant was grown in MM with Rif and Km for 2 d at 28°C with a shaking of 160 rpm. Next, after measurement of absorbance reading (600 nm) and adjustment of cell density if necessary, 1 ml of the above culture was added to 250 ml conical flask containing 50 ml of MM with Rif and Km for incubation at 28°C with shaking at 160 rpm. After 72-h cultivation, the culture supernatant was harvested with a centrifugation at 5 000 rcf for 5 min at 4°C. Then, the total RNA was extracted using an RNAiso Plus (Total RNA extraction reagent) kit (Sangon, Shanghai, China). RNA integrity was determined based on OD 260 nm /OD 280 nm ratio (>1.95), and 500 ng of DNA-free RNA with high-quality was reversely transcribed to cDNA in a 10 μl volume using PrimeScript RT Master Mix (Perfect Real Time) kit. After appropriate dilution, Table 6. Primers for the amplification of full length genes of sdmt, kari and nhad.

Primers
Oligonucleotide sequences Restriction sites b the cDNA was used for amplification of 108 bp lao gene fragment with primer set of laoF (5'-ATACGCCAAGTGCCTCAGTG-3') and laoR (5'-TCCGTCAGCCCGTTAAAGTC-3') by using the SYBR green (Tli RNaseH Plus) kit. The PCR was run on CFX Connect Real-Time System (Bio-Rad, Hercules, CA) with an amplification protocol consisting of an initial denaturation at 95°C for 10 min, followed by 40 cycles of denaturation at 95°C for 15 s and annealing/ elongation at 60°C for 30 s. Immediately after the final PCR cycle, a melting-curve analysis was made to determine the reaction specificity based on the observation of melting temperature from product. Unless otherwise specified, all the kits above were purchased from TaKaRa (Dalian, China). The cycle threshold (C T ) for each PCR was determined using STATVIEW software which automatically set the threshold signal at the log phase of the amplification curve. Several dilutions of each cDNA sample were assayed for gene of interest in order to obtain a linear regression between C T value (ranging from 10 to 30 cycles) and log of the cDNA. The amplification efficiency of gene was retrieved from the slope of that linear regression according to the formula E = 10 (−1/slope) . The 116 bp of housekeeping 16S rRNA gene fragment (access no. KP234252 in GenBank) was amplified using primer set of 16SF (5'-AAGAAGCACCGGCTAACTCC-3') and 16SR (5'-TCTCGCTTAATCAACCGCCT-3') and treated as the internal control to verify that there were equal amounts of target cDNA in all samples. The relative expression (RE) of target gene (TG) in mutant or complon compared to that in wild type Rf-1 (WT) was calculated by the comparative C T method [43]. In brief, the difference of C T between TG and reference 16S rRNA gene (RG) was calculated according to the formula: DC TðTGÞ ¼ C TðTGÞ À C TðRGÞ Then, the RE of TG compared to RG was obtained by the equation: Finally, the RE of TG in mutant or complon compared to that in WT was achieved as below: RE ¼ 2 ÀDC TðTG; Mutant or ComplonÞ =2 ÀDC TðTG; WTÞ For each experiment, triplicate reactions were performed. All Data are presented as mean ± standard error of the mean. Significance of mean difference of relative gene expression was statistically analyzed by ANOVA.
Supporting Information S1 Dataset. Expression level of 16S rRNA gene and lao in mutants and wild type strain Rf-1.