Molecular Cloning of cpcU and Heterodimeric Bilin Lyase Activity Analysis of CpcU and CpcS for Attachment of Phycocyanobilin to Cys-82 on the β-Subunit of Phycocyanin in Arthrospira platensis FACHB314

A new bilin lyase gene cpcU was cloned from Arthrospira platensis FACHB314 to study the assembly of the phycocyanin β-Subunit. Two recombinant plasmids, one contained the phycocyanobilin (PCB) producing genes (hoxI and pcyA), while the other contained the gene of the β-Subunit of phycobiliprotein (cpcB) and the lyase gene (cpcU, cpcS, or cpcU/S) were constructed and separately transferred into Escherichia coli in order to test the activities of relevant lyases for catalyzing PCB addition to CpcB during synthesizing fluorescent β-PC of A. platensis FACHB314. The fluorescence intensity examination showed that Cys-82 maybe the active site for the β-Subunit binding to PCBs and the attachment could be carried out by CpcU, CpcS, or co-expressed cpcU/S in A. platensis FACHB314.


Introduction
Phycobilisomes (PBSs) are multimeric highly-organized protein complexes that widely present in cyanobacteria and red algae, which can capture the 480 nm to 650 nm light energy and transmit the absorbed light to light system II [1,2]. PBSs are composed of colored phycobiliproteins (PBPs) and non-pigmented linker proteins. All major PBPs have a common subunit organization, in which α and β-subunits form photometric heterodimers. The non-pigmented linker proteins are responsible for organize the PBPs into the PBSs and modulate their absorptions [2]. Cyanobacterial PBS is normally composed of two PBPs, phycocyanin (PC), and allophycocyanin (APC), while phycoerythrin (PE) appeared occasionally [1].

Comparative Bioinformatics Analysis of cpcU
The complete coding sequence and the deduced amino acid sequence of CpcU are shown in the Supplementary Materials ( Figure S1). The full length DNA of cpcU has 525 nucleotides with the GC content of 43.8%. The ORF, starting with the ATG at position 1 and ending with TAA at position 525, encodes a protein of 174 amino acids, with the theoretical isoelectric point of 5.30 and the predicted molecular mass of 19.2 kDa.
BLAST and homology analysis [22] revealed that the cpcU of A. platensis FACHB314 had high identity with the cpeS super family and contained the conserved motif of a chromophore lyase, including EFF, SAGKWFS, GKS, EER, PNLR, ASF, and SEIR. In the phylogenetic analysis [23] of CpeS from other algae (Figure 1), the CpcU of A. platensis FACHB314 clustered with A. platensis NIES-39 with the confidence of 100%, and was more distantly related to Synechocystis and Synechococcus.

The Construction of the Recombinant Expression Strains
Six expression vectors containing cpcB, cpcB-cpcU, cpcB(C82A)-cpcU, cpcB(C153A)-cpcU, cpcB-cpcS, and cpcB-cpcU-cpcS, respectively, were constructed and transformed into E. coli BL21 together with the vector pET-hox1-pcyA separately. Among them, the vectors containing cpcB, cpcB-cpcU, cpcB-cpcS and cpcB-cpcU-cpcS were used to study the function of CpcU. The vectors containing cpcB(C82A)-cpcU, cpcB(C153A)-cpcU were designed to mutate the amino acid Cys at the sites 82 and 153 of the β-subunit to Ala due to the different characteristics of Cys and Ala, which was used to examine the action site in the phycobiliprotein's β-subunit catalyzed by CpcU in A. platensis FACHB314. According to the study of Shen in 2004, in Synechococcus sp. PCC 7002, the β-subunit of wild PC has two sites, the cysteine-82 and cysteine-153, which can bind PCB [8]. All the transformed strains were verified by PCR and sequencing to confirm that the inserted genes cpcB, cpcU, cpcS, and hox1-pcyA were present in the cells and the expression cassette was correct.

Expression of the Recombinant Proteins
In comparison with the control (E. coli BL21) which was grey-white color, the recombinant stains showed different degrees of blue-green color ( Figure 2). The result showed that the recombinant β-PC was expressed and attached with PCB successfully. Recombinant stain B also has the blue-green color, which suggests that the β-subunit of PC has autocatalytic activity for PCB attachment. The intensity of blue-green color of BU was higher than that of B, which may indicate that lyase CpcU has an activity in catalyzing attachment of PCB to β-PC. B(C153A)U and BU had nearly identical blue-green color, however, B(C82A)U was somewhat lighter in color compared to BU.

The Construction of the Recombinant Expression Strains
Six expression vectors containing cpcB, cpcB-cpcU, cpcB(C82A)-cpcU, cpcB(C153A)-cpcU, cpcB-cpcS, and cpcB-cpcU-cpcS, respectively, were constructed and transformed into E. coli BL21 together with the vector pET-hox1-pcyA separately. Among them, the vectors containing cpcB, cpcB-cpcU, cpcB-cpcS and cpcB-cpcU-cpcS were used to study the function of CpcU. The vectors containing cpcB(C82A)-cpcU, cpcB(C153A)-cpcU were designed to mutate the amino acid Cys at the sites 82 and 153 of the β-subunit to Ala due to the different characteristics of Cys and Ala, which was used to examine the action site in the phycobiliprotein's β-subunit catalyzed by CpcU in A. platensis FACHB314. According to the study of Shen in 2004, in Synechococcus sp. PCC 7002, the β-subunit of wild PC has two sites, the cysteine-82 and cysteine-153, which can bind PCB [8]. All the transformed strains were verified by PCR and sequencing to confirm that the inserted genes cpcB, cpcU, cpcS, and hox1-pcyA were present in the cells and the expression cassette was correct.

Expression of the Recombinant Proteins
In comparison with the control (E. coli BL21) which was grey-white color, the recombinant stains showed different degrees of blue-green color ( Figure 2). The result showed that the recombinant β-PC was expressed and attached with PCB successfully. Recombinant stain B also has the blue-green color, which suggests that the β-subunit of PC has autocatalytic activity for PCB attachment. The intensity of blue-green color of BU was higher than that of B, which may indicate that lyase CpcU has an activity in catalyzing attachment of PCB to β-PC. B(C153A)U and BU had nearly identical blue-green color, however, B(C82A)U was somewhat lighter in color compared to BU.

The Construction of the Recombinant Expression Strains
Six expression vectors containing cpcB, cpcB-cpcU, cpcB(C82A)-cpcU, cpcB(C153A)-cpcU, cpcB-cpcS, and cpcB-cpcU-cpcS, respectively, were constructed and transformed into E. coli BL21 together with the vector pET-hox1-pcyA separately. Among them, the vectors containing cpcB, cpcB-cpcU, cpcB-cpcS and cpcB-cpcU-cpcS were used to study the function of CpcU. The vectors containing cpcB(C82A)-cpcU, cpcB(C153A)-cpcU were designed to mutate the amino acid Cys at the sites 82 and 153 of the β-subunit to Ala due to the different characteristics of Cys and Ala, which was used to examine the action site in the phycobiliprotein's β-subunit catalyzed by CpcU in A. platensis FACHB314. According to the study of Shen in 2004, in Synechococcus sp. PCC 7002, the β-subunit of wild PC has two sites, the cysteine-82 and cysteine-153, which can bind PCB [8]. All the transformed strains were verified by PCR and sequencing to confirm that the inserted genes cpcB, cpcU, cpcS, and hox1-pcyA were present in the cells and the expression cassette was correct.

Expression of the Recombinant Proteins
In comparison with the control (E. coli BL21) which was grey-white color, the recombinant stains showed different degrees of blue-green color ( Figure 2). The result showed that the recombinant β-PC was expressed and attached with PCB successfully. Recombinant stain B also has the blue-green color, which suggests that the β-subunit of PC has autocatalytic activity for PCB attachment. The intensity of blue-green color of BU was higher than that of B, which may indicate that lyase CpcU has an activity in catalyzing attachment of PCB to β-PC. B(C153A)U and BU had nearly identical blue-green color, however, B(C82A)U was somewhat lighter in color compared to BU.

Fluorescence Emission Spectra
The cell suspensions of recombinant strains were used to check the specific PC fluorescence emission spectra after excitation at 580 nm ( Figure 4). All samples have been measured for three times and all of the data were analyzed by using statistical analysis method. After calculation of the fluorescence intensity of the unit concentration of phycocyanin (Tables 1 and 2), the result showed that the spectrum of control E. coli BL21 was smooth, while the recombinant strains B, BU, BS, BUS, B(C82A)U, and B(153A)U all have a peak of fluorescence emission at about 633 nm, which verified the successful expression of the transformed genes and the attachment of PCB onto apo-PC. The recombinant strain B also showed fluorescence characteristics of PC, suggesting that β-PC has autocatalytic activity for the attachment with PCB. The recombinant strain BU shows a higher fluorescence intensity than that of the strain B ( Figure 4A) and the difference is significant (p < 0.05). In addition, the fluorescence intensity of the strain BU seems higher than that of the recombinant strains BUS and BS ( Figure 4A), but the difference is not significant (p > 0.05). BUS has the similar fluorescence intensity with BS. The result indicated that in A. platensis FACHB314, CpcU, and CpcS had the chromophore lyase function separately and did not show the coordination effect. B(C82A)U and B(153A)U both have a peak of fluorescence emission at about 633 nm; B(C82A)U almost has the same high fluorescence intensity with BU, while the peak of B(C82A)U is much lower than B(C153A)U ( Figure 4B), which indicated that Cys-82 may be the active site of the β subunit catalyzed by CpcU to bind to phycocyanobilins in A. platensis FACHB314.

Fluorescence Emission Spectra
The cell suspensions of recombinant strains were used to check the specific PC fluorescence emission spectra after excitation at 580 nm ( Figure 4). All samples have been measured for three times and all of the data were analyzed by using statistical analysis method. After calculation of the fluorescence intensity of the unit concentration of phycocyanin (Tables 1 and 2), the result showed that the spectrum of control E. coli BL21 was smooth, while the recombinant strains B, BU, BS, BUS, B(C82A)U, and B(153A)U all have a peak of fluorescence emission at about 633 nm, which verified the successful expression of the transformed genes and the attachment of PCB onto apo-PC. The recombinant strain B also showed fluorescence characteristics of PC, suggesting that β-PC has autocatalytic activity for the attachment with PCB. The recombinant strain BU shows a higher fluorescence intensity than that of the strain B ( Figure 4A) and the difference is significant (p < 0.05). In addition, the fluorescence intensity of the strain BU seems higher than that of the recombinant strains BUS and BS ( Figure 4A), but the difference is not significant (p > 0.05). BUS has the similar fluorescence intensity with BS. The result indicated that in A. platensis FACHB314, CpcU, and CpcS had the chromophore lyase function separately and did not show the coordination effect. B(C82A)U and B(153A)U both have a peak of fluorescence emission at about 633 nm; B(C82A)U almost has the same high fluorescence intensity with BU, while the peak of B(C82A)U is much lower than B(C153A)U ( Figure 4B), which indicated that Cys-82 may be the active site of the β-subunit catalyzed by CpcU to bind to phycocyanobilins in A. platensis FACHB314.

Discussion
In this study, a chromophore bilin lyase gene cpcU of phycocyanin β subunit was first cloned from A. platensis FACHB314. The result of homology searches using the BLAST program show that CpcU is a relatively conserved protein in cyanobacteria, which has seven conserved domains including EFF, SAGKWFS, GKS, EER, PNLR, ASF, and SEIR (Supplementary Materials). CpcU and CpcS (FO818640.1) both are belong to CpeS superfamily by amino acid blasting, and Figure 5 shows that their similarity reaches to 29.8%. By multiple sequence alignment of CpcU with other cyanobacteria, two conserved amino acid tryptophan coding sites (14 and 142) were found, and the conservative tryptophan residues also exist in CpcS. We speculate that these two tryptophans may play an important role for chromophore lyase to exert its catalytic activity, and CpcU may have the similar chromophore lyase activity with the CpeS. To confirm this speculation, two recombinants were constructed to study and compare the function of the CpcU. In the recombinants, two polarity Cys at the 82 and 153 sites of phycocyanin β subunit were mutated to a non-polar-alanine (Ala) to study the working site of CpcU on phycocyanin β subunit. The results of SDS-PAGE and Western blotting showed that the mutant strain can also express phycocyanin, but the result of fluorescence spectra testing appeared that the fluorescence intensity of Cys 82 -mutant strains was lower than that of the non-mutated strain, while the fluorescence intensity of Cys 153 -mutant strain was almost equal with the non-mutated strain ( Figure 4A). Based on these, we speculate that CpcU has an effect on the cysteine residue of the 82 site in phycocyanin β subunit, which was the same with the activity site of CpcS.

Discussion
In this study, a chromophore bilin lyase gene cpcU of phycocyanin β-subunit was first cloned from A. platensis FACHB314. The result of homology searches using the BLAST program show that CpcU is a relatively conserved protein in cyanobacteria, which has seven conserved domains including EFF, SAGKWFS, GKS, EER, PNLR, ASF, and SEIR (Supplementary Materials). CpcU and CpcS (FO818640.1) both are belong to CpeS superfamily by amino acid blasting, and Figure 5 shows that their similarity reaches to 29.8%. By multiple sequence alignment of CpcU with other cyanobacteria, two conserved amino acid tryptophan coding sites (14 and 142) were found, and the conservative tryptophan residues also exist in CpcS. We speculate that these two tryptophans may play an important role for chromophore lyase to exert its catalytic activity, and CpcU may have the similar chromophore lyase activity with the CpeS. To confirm this speculation, two recombinants were constructed to study and compare the function of the CpcU. In the recombinants, two polarity Cys at the 82 and 153 sites of phycocyanin β-subunit were mutated to a non-polar-alanine (Ala) to study the working site of CpcU on phycocyanin β-subunit. The results of SDS-PAGE and Western blotting showed that the mutant strain can also express phycocyanin, but the result of fluorescence spectra testing appeared that the fluorescence intensity of Cys 82 -mutant strains was lower than that of the non-mutated strain, while the fluorescence intensity of Cys 153 -mutant strain was almost equal with the non-mutated strain ( Figure 4A). Based on these, we speculate that CpcU has an effect on the cysteine residue of the 82 site in phycocyanin β-subunit, which was the same with the activity site of CpcS.

Discussion
In this study, a chromophore bilin lyase gene cpcU of phycocyanin β subunit was first cloned from A. platensis FACHB314. The result of homology searches using the BLAST program show that CpcU is a relatively conserved protein in cyanobacteria, which has seven conserved domains including EFF, SAGKWFS, GKS, EER, PNLR, ASF, and SEIR (Supplementary Materials). CpcU and CpcS (FO818640.1) both are belong to CpeS superfamily by amino acid blasting, and Figure 5 shows that their similarity reaches to 29.8%. By multiple sequence alignment of CpcU with other cyanobacteria, two conserved amino acid tryptophan coding sites (14 and 142) were found, and the conservative tryptophan residues also exist in CpcS. We speculate that these two tryptophans may play an important role for chromophore lyase to exert its catalytic activity, and CpcU may have the similar chromophore lyase activity with the CpeS. To confirm this speculation, two recombinants were constructed to study and compare the function of the CpcU. In the recombinants, two polarity Cys at the 82 and 153 sites of phycocyanin β subunit were mutated to a non-polar-alanine (Ala) to study the working site of CpcU on phycocyanin β subunit. The results of SDS-PAGE and Western blotting showed that the mutant strain can also express phycocyanin, but the result of fluorescence spectra testing appeared that the fluorescence intensity of Cys 82 -mutant strains was lower than that of the non-mutated strain, while the fluorescence intensity of Cys 153 -mutant strain was almost equal with the non-mutated strain ( Figure 4A). Based on these, we speculate that CpcU has an effect on the cysteine residue of the 82 site in phycocyanin β subunit, which was the same with the activity site of CpcS.  According to the report, whether in the cyanobacteria or in the heterologous host, once PCB was correctly ligated to apo-PC, its specific blue-green color and fluorescence spectrum should be detectable. Recombinant strains constructed in this research all appeared blue-green in color and present the specific fluorescence spectrum of PC. Recombinant strain B shows a relatively high intensity of fluorescence, suggesting that CpcB is able to attach PCB onto itself, spontaneously. Recombinant strains BU and BS show the higher fluorescence intensity than strain B, which suggests that both CpcU and CpcS have the function to attach PCB to β-PC. The fluorescence intensity of the recombinant strain BUS is between BU and BS, which indicates that there is no coordination effect between CpcU and CpcS in A. platensis FACHB314. Among the three strains of BU, BS, and BUS, BU shows the highest fluorescence intensity, which indicates that CpcU may work alone and play an important role in specific covalent attachment of PCB on the Cys-82 of β-PC. This result differs from those obtained in Nostoc sp. PCC7120. [11], in which only the product of CpeS was required for PCB addition to Cys-82 of β-PC. It is unclear why these two lyase subunits are required for some cyanobacteria, but not for others. According to the phylogenetic analyses, the Nostoc sp. PCC7120 belongs to a phylogenetically distinct subgroup of the CpcS-III. Whether organisms with CpcS-III arose by the loss of CpcU or organisms with cpcS-I gained cpcU by a gene duplication event is presently unclear.
According to the fluorescence spectra of recombinant strains, BU, BS, and BUS showed the same emission peak at 636 nm, with an 8 nm blue-shift from the native PC (λ max = 644 nm). Such a blue-shift may be related to the change in chemical structure of PBPs. In wild-type strains, PC is composed of two subunits (αβ) but usually exists as a trimer (αβ) 3 or a hexamer (αβ) 6 [6,24]. In this study, only β-PC was expressed in E. coli and, thus, no integrated PC could be constructed. The absorption and emission peaks of the monomer are blue-shifted more than the trimmers, which is consistent with the report by MacColl et al. [25].

Strains and Plasmids
The plasmid pET-hox1-pcyA was constructed to contain genes hox1 and pcyA which were cloned from A. platensis FACHB314. These two genes could express enzymes catalyze heme into phycocyanobilins (PCB) in E. coli. The plasmid pACYCDuet-cpcB contains gene cpcB, encoding β-PC. The plasmid pACYCDuet-cpcB-cpcS contains genes cpcB and cpcS, among them, cpcS could express a chromophore lyase of A. platensis FACHB314 ( Figure 6). All of the strains and plasmids used in this study are listed in Table 3. According to the report, whether in the cyanobacteria or in the heterologous host, once PCB was correctly ligated to apo-PC, its specific blue-green color and fluorescence spectrum should be detectable. Recombinant strains constructed in this research all appeared blue-green in color and present the specific fluorescence spectrum of PC. Recombinant strain B shows a relatively high intensity of fluorescence, suggesting that CpcB is able to attach PCB onto itself, spontaneously. Recombinant strains BU and BS show the higher fluorescence intensity than strain B, which suggests that both CpcU and CpcS have the function to attach PCB to β-PC. The fluorescence intensity of the recombinant strain BUS is between BU and BS, which indicates that there is no coordination effect between CpcU and CpcS in A. platensis FACHB314. Among the three strains of BU, BS, and BUS, BU shows the highest fluorescence intensity, which indicates that CpcU may work alone and play an important role in specific covalent attachment of PCB on the Cys-82 of β-PC. This result differs from those obtained in Nostoc sp. PCC7120. [11], in which only the product of CpeS was required for PCB addition to Cys-82 of β-PC. It is unclear why these two lyase subunits are required for some cyanobacteria, but not for others. According to the phylogenetic analyses, the Nostoc sp. PCC7120 belongs to a phylogenetically distinct subgroup of the CpcS-III. Whether organisms with CpcS-III arose by the loss of CpcU or organisms with cpcS-I gained cpcU by a gene duplication event is presently unclear.
According to the fluorescence spectra of recombinant strains, BU, BS, and BUS showed the same emission peak at 636 nm, with an 8 nm blue-shift from the native PC (λmax = 644 nm). Such a blue-shift may be related to the change in chemical structure of PBPs. In wild-type strains, PC is composed of two subunits (αβ) but usually exists as a trimer (αβ)3 or a hexamer (αβ)6 [6,24]. In this study, only β-PC was expressed in E. coli and, thus, no integrated PC could be constructed. The absorption and emission peaks of the monomer are blue-shifted more than the trimmers, which is consistent with the report by MacColl et al. [25].

Strains and Plasmids
The plasmid pET-hox1-pcyA was constructed to contain genes hox1 and pcyA which were cloned from A. platensis FACHB314. These two genes could express enzymes catalyze heme into phycocyanobilins (PCB) in E. coli. The plasmid pACYCDuet-cpcB contains gene cpcB, encoding β-PC. The plasmid pACYCDuet-cpcB-cpcS contains genes cpcB and cpcS, among them, cpcS could express a chromophore lyase of A. platensis FACHB314 ( Figure 6). All of the strains and plasmids used in this study are listed in Table 3.

Genomic DNA Isolation and Gene Cloning of cpcU
A. platensis FACHB314 was cultured in Zarrouk medium at 25 °C in our laboratory and its genomic DNA was extracted by using the Universal Genomic DNA Extraction kit (TaKaRa, Dalian, China).
According The restriction enzyme sites NdeI and BglII (underlined in the primer sequences) were incorporated at the 5' ends of the primers to be used to digest and ligate the cpcU into the expression vector. The cpcU gene was amplified by PCR with the DNA of A. platensis FACHB314 as the template and the primers cpcU-F and cpcU-R. After being sequenced and blasted with the sequence in the GenBank, the PCR product was verified to be the cpcU preliminary.

Construction of the Recombinant Expression Vectors
The cpcU was double-digested with the restriction enzymes NdeI and BglII and inserted into the vector pACYCDuet-cpcB to produce the expression vector pACYCDuet-cpcB-cpcU. Then the vector pACYCDuet-cpcB-cpcU was transformed into the E. coli DH5α competent cell. After cultivation on the Luria-Bertani (LB) solid medium plate with chloramphenicol (34 μg•mL −1 ), the positive clone was screened and verified by sequencing.
The plasmid pACYCDuet-cpcB-cpcS was extracted from recombinant strain BS using the High Pure Plasmid Extraction kit (Biomed, Beijing, China). The plasmid was digested by the restriction enzymes AatII and KpnI, and then ligated with the fragment cpcU, to yield the expression vector pACYCDuet-cpcB-cpcU-cpcS.
To study the ligation site of the β subunit with the PCB catalyzed by chromophore lyase CpcU, site-directed mutagenesis was used to mutate the amino acid Cys at the sites 82 and 153 of the  , primers (cpcU-F: 5 1 -GGAATTCCATATGATGGATATTGTCG AATTTTTTGAGTTG-3 1 , cpcU-R: 5 1 -GGAAGATCTTTACGTTAAAC CATGCGAATTTC -3 1 ) were designed based on the conserved sequences. The restriction enzyme sites NdeI and BglII (underlined in the primer sequences) were incorporated at the 5' ends of the primers to be used to digest and ligate the cpcU into the expression vector. The cpcU gene was amplified by PCR with the DNA of A. platensis FACHB314 as the template and the primers cpcU-F and cpcU-R. After being sequenced and blasted with the sequence in the GenBank, the PCR product was verified to be the cpcU preliminary.

Construction of the Recombinant Expression Vectors
The cpcU was double-digested with the restriction enzymes NdeI and BglII and inserted into the vector pACYCDuet-cpcB to produce the expression vector pACYCDuet-cpcB-cpcU. Then the vector pACYCDuet-cpcB-cpcU was transformed into the E. coli DH5α competent cell. After cultivation on the Luria-Bertani (LB) solid medium plate with chloramphenicol (34 µg¨mL´1), the positive clone was screened and verified by sequencing.
The plasmid pACYCDuet-cpcB-cpcS was extracted from recombinant strain BS using the High Pure Plasmid Extraction kit (Biomed, Beijing, China). The plasmid was digested by the restriction enzymes AatII and KpnI, and then ligated with the fragment cpcU, to yield the expression vector pACYCDuet-cpcB-cpcU-cpcS.
To study the ligation site of the β-subunit with the PCB catalyzed by chromophore lyase CpcU, site-directed mutagenesis was used to mutate the amino acid Cys at the sites 82 and 153 of the β-subunit to Ala due to the different characteristics of Cys and Ala. By analyzing the preferred codons of A. platensis FACHB314, the codon for Ala should be GCT. So to mutate the amino acids Cys-82 and Cys-153 of cpcB to Ala, four primers were designed as follows: cpcB82-F5'-CGTCG TATGGCTGCTGCTTTGCG-3 1 , cpcB82-R5'-TGACATGGAAATCATCCTGCGCTATG-3 1 , cpcB153-F5'-GTATCACTCCTGGTGATGCTAGCGC-3 1 , and cpcB153-R5'-TTTGGCTTCAGAAATCGCTGGTTAC TTTG-3 1 . Using the vector pACYCDuet-cpcB-cpcU as the template, the site-directed mutated DNA was obtained by PCR amplification using the Mutation Kit (TaKaRa). The mutated linear DNA was annularly connected using the DNA Blunting Kit (TaKaRa), and transformed into E. coli DH5α. The transformants were screened on Luria-Bertani (LB) plates containing 34 µg¨mL´1 of chloramphenicol (Cm) and verified by sequencing.

Plasmid Transformation and Protein Expression
Six recombinant expression plasmids (pACYCDuet-cpcB, pACYCDuet-cpcB-cpcU, pACYCDuet-cpcB(C82A)-cpcU, pACYCDuet-cpcB(C153A)-cpcU, pACYCDuet-cpcB-cpcS, and pACYCDuet-cpcB-cpcU-cpcS) were transformed into E. coli BL21 with pET-hox1-pcyA to produce the recombinant E. coli strains, including B, BU, B(C82A)U, B(C153A)U, BS, and BUS (Table 4). Positive colonies were selected on LB medium plates with the presence of 34 µg¨mL´1 chloramphenicol (Cm) and 100 µg¨mL´1 kanamycin (Km), and then confirmed by PCR amplification of the inserted genes. For expression of the recombinant protein in the transformed strains, 2.5 mL starter culture cells were added into 250 mL LB medium with the antibiotics Cm and Km and shaken at 37˝C until the optical density at 600 nm (OD 600 ) was 0.6. Production of the proteins was induced by the addition of 0.1 mM isopropyl-β-D-thiogalactoside (IPTG). Cells were incubated with shaking at 200 rpm at 37˝C for 3 h and the OD 600 was measured again to ensure that the cell densities were the same before they were harvested by centrifugation at 4000 g for 25 min. Cell pellets were rinsed twice with 0.9% NaCl and then resuspended in 3 mL 0.1 M PBS buffer (pH 7.2). After ultrasonically lysed on ice for 6 min, cell suspensions were centrifuged at 12,000 g for 15 min and the supernatants were used for SDS-PAGE, Western blotting analysis and fluorescence emission spectra detection.

Recombinant Protein Analysis
Protein fractions were analyzed by polyacrylamide gel electrophoresis with the presence of SDS [10,22,23]. SDS-PAGE gel was made with 15% separation gel and 5% stacking gel (MDBio, Taiwan, China). Cells of the expression strains were lysed by ultrasonic disruption and centrifuged, and then the supernatant was boiled with 5ˆbuffer before loading. The resolved proteins were visualized by staining with Coomassie Blue. Launch SensiAnsys was used for quantitative analysis of the percentage of the phycocyanin in the total protein. Then, the quantity of expressed recombinant phycocyanin was calculated by multiply the percentage of phycocyanin in the total protein and the total protein concentration. The total protein concentration was measured using a NANODROP 2000C spectrophotometer. Western blotting analysis was performed using the c-phycocyanin (C-PC) antibody as the primary antibody and peroxidase-conjugated goat anti-rabbit IgG as the secondary antibody.
The hybridization bands in the nitrocellulose membrane were observed to confirm the expression of phycocyanin.

Fluorescence Emission Spectra
The fluorescence emission spectra for each sample by using a fluorescence spectrophotometer (HITACHI F-4600) excited at 580 nm. The quantity of each sample used for detection was 1 mL and all samples have been measured three times. The excitation and emission slit width was set at 10 nm with a scan speed of 1200 nm/min. To analyze the function of CpcU, the fluorescence intensity of the different strains should be compared. Thus, the fluorescence intensity per unit mass of recombinant phycocyanin was calculated by the ratio of the fluorescence intensity at the highest emission peak and the concentration of phycocyanin [13].

Conclusions
The present work has cloned a bilin lyase gene cpcU in Arthrospira platensis FACHB314 and the CpcU was confirmed to have the function to attach PCB to Cys-82 on β-PC. In our previous work, CpcS were found to attach PCB to Cys-82 on β-PC, and CpcT could attach PCB to Cys-153 on β-PC in A. platensis FACHB314. Compared with CpcT, the catalytic activity of CpcU and CpcS are weaker.