Cloning, Sequencing, and Expression in Escherichia coli of the New Gene Encoding beta -1,3-Xylanase from a Marine Bacterium, Vibrio sp. Strain XY-214

doi:10.1128/AEM.66.4.1741-1743.2000

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Applied and Environmental Microbiology, April 2000, p. 1741-1743, Vol. 66, No. 4
0099-2240/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Cloning, Sequencing, and Expression in Escherichia coli of the New Gene Encoding $beta$ -1,3-Xylanase from a Marine Bacterium, Vibrio sp. Strain XY-214

Toshiyoshi Araki,^* Shinnosuke Hashikawa, and Tatsuo Morishita

Faculty of Bioresources, Mie University, Kamihama, Tsu, Mie 514-8507, Japan

Received 8 September 1999/Accepted 19 January 2000

	ABSTRACT

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The Vibrio sp. strain XY-214 $beta$ -1,3-xylanase gene cloned in Escherichia coli DH5 $alpha$ consisted of an open reading frame of 1,383nucleotides encoding a protein of 460 amino acids with a molecularmass of 51,323 Da and had a signal peptide of 22 amino acids.The transformant enzyme hydrolyzed $beta$ -1,3-xylan to produce severalxylooligosaccharides.

	TEXT

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$beta$ -1,3-Xylan is a homopolymer of $beta$ -1,3-linked D-xylose and is a polysaccharide peculiar to marine algae; it is contained inthe cell walls of red algae (Porphyra and Bangia) and green algae(Caulerupa, Bryopsis, and Udotea) (9, 13). $beta$ -1,3-Xylanase(1,3- $beta$ -D-xylan xylanohydrolase; EC 3.2.1.32) is a $beta$ -1,3-xylan-hydrolyzingenzyme that is useful for structural analysis of the cell wallsof these algae and for protoplast isolation, which is an importanttechnique for cell fusion and gene manipulation of algae. On theother hand, $beta$ -1,4-xylan is a major component of hemicellulosesof land plant cell walls (19). $beta$ -1,4-Xylanases (1,4- $beta$ -D-xylanxylanohydrolase; EC 3.2.1.8) are produced by many kinds of microorganisms,including aerobic and anaerobic mesophiles and thermophiles, andtheir biochemical and molecular characteristics have been widelystudied (6, 14, 15). Compared with $beta$ -1,4-xylanase, therehave been only a few reports on enzymatic studies of $beta$ -1,3-xylanasebased on three bacteria, Vibrio sp. strain AX-4 (1), Pseudomonassp. strain PT-5 (21), and Alcaligenes sp. strain XY-234 (2),as well as one fungus, Aspergillus terreus A-07 (7). Hernandezet al. have only recently entered data on sequencing of the $beta$ -1,3-xylanasegene in the DDBJ/EMBL/GenBank database (A. Hernandez, J. C. Lopez,J. L. Copa-Patino, and T. Soliveri, unpublished data. [DDBJ/EMBL/GenBankaccession no. AF121865]).

We have purified $beta$ -1,3-xylanase from Vibrio sp. strain XY-214 isolated from a marine environment and characterized its properties(3). In this paper, we describe the cloning and DNA sequencingof the $beta$ -1,3-xylanase gene (txyA) of Vibrio sp. strain XY-214and its expression in Escherichia coli.

Construction of the probe for cloning of the txyA gene. $beta$ -1,3-Xylanase was purified according to a previously described procedure (3). After the purified enzyme was digested witha sequencing grade-modified trypsin (Promega, Madison, Wis.),the tryptic digest was fractionated by high-performance liquidchromatography (µ Bondsphere, 300 Å, C₁₈, 3.9 by 150 mm; Waters).The 16th peak (peptide 16) out of 33 peaks separated was collectedand blotted onto a glass filter treated with Bio Brene Plus (AppliedBiosystems, Foster City, Calif.). The N-terminal amino acid sequencewas determined by automated Edman sequencing on a model 473A gas-phasesequencer (AppliedBiosystems).

The degenerate primers (primers F and R) were designed on the basis of the underlined parts of the N-terminal amino acid sequencesof the purified $beta$ -1,3-xylanase (sequence LDGKLVPDQGILVSVGQDV)and peptide 16 (sequence WAAPYNEGYWGDSR). The alignment of primerF is GAYGGNAARTTIGTNCCNGA, and that of primer R is CCCCARTNACCYTCRTTRTA,where Y, R, I, and N indicate C or T, A or G, inosine, and anynucleotides, respectively. For construction of the probe for cloningof txyA, one specifically amplified oligonucleotide was obtainedfrom a template of genomic DNA of Vibrio sp. strain XY-214 byPCR with the degenerate primers (F and R). The PCR product ligatedinto pUC19-T vector (12) was composed of 860 bp encoding 286amino acid residues. The sequences of the first seven N-terminaland the last six C-terminal amino acids of the fragment were confirmedto be identical to the amino acid sequence of native $beta$ -1,3-xylanaseand peptide 16. Therefore, the DNA insert in pUC19-T vector wasconsidered to be derived from the gene encoding $beta$ -1,3-xylanaseand was used as the probe forcloning.

Cloning of the txyA gene. Genomic DNA was conferred by double digestion with two enzymes (BglII and XbaI), and fragments of about 4.4 kbp, which weredeemed to be a suitable size considering the molecular mass ofthe enzyme, were selected as positive on an alkaline phosphatase-labeledprobe. When BglII-XbaI fragments were ligated into pBluescriptII KS( $-$ ) and transformed into E. coli DH5 $alpha$ , 22 of the 860 cloneshybridized to the alkaline phosphatase-labeled probe. The recombinantplasmid yielded from 1 of the 22 clones was termedpTXY1.

Analysis of DNA sequence. The pTXY1 was digested singly with three restriction enzymes (EcoRV, HindIII and KpnI), and the fragments were subcloned intopBluescript II KS( $-$ ) vector. The subcloned fragments, togetherwith T3 and T7 primers and some synthetic primers, were used tosequence the entire BglII-XbaI fragment (ca. 4.4 kbp). The nucleotidesequences of both strands of the subcloned DNA inserts were determinedwith an Applied Biosystems model 373A automated DNA sequencer(Applied Biosystems). The nucleotide sequence data of the fragmentappear in the DDBJ/EMBL/GenBank nucleotide sequence databasesunder the accession no. AB029043.

The insert in pTXY1 was found to have one complete open reading frame (ORF-2), which was placed between two incomplete ORFs(ORF-1 of 2,268 bp and ORF-3 of 504 bp). The amino acid sequencesof positions 23 (Leu) to 41 (Var) and 300 (Trp) to 313 (Arg) inORF-2 coincided with the N-terminal amino acid sequences of native $beta$ -1,3-xylanase and peptide 16, respectively. Therefore, ORF-2,extending from position 2457 to position 3839, was estimated tocode for the txyA gene of Vibrio sp. strain XY-214. The txyA genewas composed of 1,383 bp encoding 460 amino acid residues witha molecular mass of 51,323 Da and was found to contain a signalpeptide consisting of 22 amino acids from the first methionine.The signal peptide exhibited the structural features of a signalpeptide which is known generally to possess a few positively chargedresidues, a hydrophobic core of approximately 12 amino acids,and the Ala-X-Ala sequence that is the most frequent sequencepreceding signal peptidase cleavage (16, 20). Thus, afterprocessing of the signal peptide, the molecular mass of the matureenzyme seems to be composed of 438 amino acids comprising a molecularmass of 49,050 Da. The 103-nucleotide region between the translationinitiation codon (ATG) of ORF-2 and the first palindrome (2,277to 2,308 bp) structure upstream from it was large enough for thepromoter. A putative ribosome-binding site sequence (AGGAAG) islocated 13 nucleotides upstream from the initiation codon. Putativepromoter sequences of the $-$ 10 region (TTTAAT) and $-$ 35 region (TTGTTC)were found 28 and 47 bp upstream from the initial codon, respectively.The palindromic sequence located 24 bp downstream of the stopcodon could form an mRNA hairpin loop with a $Delta$ G of $-$ 15.4 kcal/mol(ca. $-$ 64.4 kJ/mol) (11) and might act as a signal for transcriptiontermination of a rho-independentpromoter.

ORF-2 was in the opposite orientation to the LacZ promoter of pBluescript, and the transformant E. coli DH5 $alpha$ strain harboringpTXY1 exhibited $beta$ -1,3-xylanase activity when grown in culturemedium supplemented with or without IPTG (isopropyl- $beta$ -D-thiogalactopyranoside).Therefore, the txyA gene in pTXY1 was found to be able to expressthe enzyme activity by using its ownpromoter.

Homology. The deduced amino acid sequence (460 residues) of $beta$ -1,3-xylanase from Vibrio sp. strain XY-214 was compared with entries inthe Blast sequence databases. The only glycoside hydrolase havinghigh homology with Vibrio sp. strain XY-214 $beta$ -1,3-xylanase wasthe mannosidase from Thermotoga neapolitana, of which the geneconsisted of 1,041 bp encoding 346 amino acids (D. A. Yernoal,S. Y. Rani, R. F. Sullivan, and D. E. Eveleigh, unpublished data[DDBJ/EMBL/GenBank accession no. U58632]); the homology betweenboth enzymes was 40.6% of their amino acidsequences.

There have been many reports on the amino acid sequences of $beta$ -1,4-xylanases, which belong to families 5, 10, 11, and 43 among77 families of glycoside hydrolase classified on the basis ofamino acid sequence similarities (8). Of the amino acid sequencesof $beta$ -1,3-xylanase, that of Streptomyces has been registered inthe database recently (A. Hernandez, J. C. Lopez, J. L. Copa-Patino,and J. Soliveri, unpublished data [DDBJ/EMBL/GenBank accessionno. AF121865]) Streptomyces $beta$ -1,3-xylanase (EC 3.2.1.32)exhibited over 80% homology to $beta$ -1,4-xylanases of some microorganismsbelonging to family 10, which includes $beta$ -1,4-xylanase (EC 3.2.1.8)and cellobiohydrolase (EC 3.2.1.91). However, the amino acidsequence of $beta$ -1,3-xylanase of Vibrio sp. strain XY-214 had only17% homology to that of Streptomyces $beta$ -1,3-xylanase. We have notobtained information on enzymatic properties other than the sequencesentered at the database on the Streptomyces $beta$ -1,3-xylanase andthe T. neapolitana mannosidase because such data have not beenpublished.

Expression of the recombinant $beta$ -1,3-xylanase from a transformant. The activity of the enzyme toward $beta$ -1,3-xylan was measured by the release of reducing sugar equivalent (18). $beta$ -1,3-Xylanwas prepared from a green alga, Caulerpa racemosa var. laetevirensaccording to the method of Iriki et al. (9). The transformantwas grown in Luria-Bertani medium containing ampicillin (3,000ml). The cells collected by centrifugation (10,000 × g, 10 min)were suspended in 70 ml of 50 mM Tris-HCl buffer (pH 7.5) anddisrupted by a sonicator. The $beta$ -1,3-xylanase activity of the supernatantcollected by centrifugation was 8.5 U, though the extracellularenzyme of Vibrio sp. strain XY-214 exhibited 400 U per 3 litersof culture fluid. The supernatant was purified by a combinationof Q Sepharose (3), $beta$ -1,3-xylan-affinity (1), and Mono Q(3) column chromatographies. As shown in Fig. 1, the finalenzyme preparation was ascertained to be homogeneous by sodiumdodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE)and exhibited $beta$ -1,3-xylanase activity by zymography. SDS-PAGEwas performed in 12.5% polyacrylamide gel by using the buffersystem of Laemmli (10). Zymography was achieved by using glycol $beta$ -1,3-xylan (17) according to the method of Beguin (5). Theactive band coincided in position with the native enzyme. Themolecular mass of the purified enzyme from the transformant was52 kDa, the same as the value determined by SDS-PAGE for the native $beta$ -1,3-xylanase from Vibrio sp. strain XY-214, but a little largerthan the value (49,050 Da) estimated from the deduced amino acidsequence of $beta$ -1,3-xylanase. However, the molecular masses of therecombinant txyA enzyme and the native enzyme were estimated tobe 48.0 and 46.4 kDa by Superdex 200 fast-protein liquid chromatographywith gel filtration, respectively, and these values were foundto be a little smaller than the value of the deduced amino acidsequence. The recombinant enzyme band separated by SDS-PAGE wastransferred onto a Clear Blot Membrane-p AE-6660 (Atto, Japan).The sequences of the first five N-terminal amino acids were determined.The sequence (LDGKL) was in a good agreement with that of thenative enzyme. As shown in Fig. 2, the recombinant enzyme hydrolyzed $beta$ -1,3-xylan to produce several xylooligosaccharides, but did notact on $beta$ -1,4-xylan, curdlan (which is a polymer of the repeatingunits of $beta$ -1,3-xylan-linked D-glucose), or carboxymethylcellulose.The latter three polysaccharides were purchased from Sigma Co.,Ltd. $beta$ -1,3-Xylan used as the substrate was not cleaved by a commercialenzyme (Macerozyme R-10 from Tricoderma; Yakult Co., Ltd.) capableof hydrolyzing $beta$ -1,4-xylan. The $beta$ -1,3-xylanase from Vibrio sp.strain XY-214 exhibited 40.6% homology with the mannosidase fromT. neapolitana (D. A. Yernool, S. Y. Rani, R. F. Sullivan, andD. E. Eveleigh, unpublished data [DDBJ/EMBL/GenBank accessionno. U58632]). However, neither $beta$ -1,3-xylanases from Vibriosp. strain XY-214 nor the recombinant E. coli showed the $alpha$ - and $beta$ -mannosidase activities (data not shown).

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FIG. 1. SDS-PAGE (A) and zymography (B) of the native and recombinant $beta$ -1,3-xylanases. (A) SDS-PAGE. Proteins (20 µg) were stained with Coomassie brilliant blue R-250. (B) Zymography. Both purified enzymes were applied to an SDS-PAGE gel, followed by activity staining with glycol $beta$ -1,3-xylan as the substrate. Numbers on the left are molecular masses of the markers. Lanes: 1, molecular mass markers; 2 and 4, native $beta$ -1,3-xylanase; 3 and 5, recombinant $beta$ -1,3-xylanase.

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FIG. 2. Thin-layer chromatogram of hydrolysis products obtained from several polysaccharides with the recombinant $beta$ -1,3-xylanase. Fifty microliters of enzyme solution (0.05 U of $beta$ -1,3-xylanase) was added to 50 µl of 10 mM sodium acetate buffer (pH 6.0) containing 1% polysaccharide and incubated at 37°C overnight. The hydrolysis products were developed on a silica gel 60 plastic sheet in a solvent of n-butanol-acetic acid-water (10:5:1), and the oligosaccharides were visualized by spraying the plate with a diphenylamine-aniline-phosphate reagent (4). Lanes: 1 and 11, D-xylose; 2, $beta$ -1,3-xylanase; 3, $beta$ -1,3-xylan; 5, $beta$ -1,4-xylan; 7, curdlan; 9, carboxymethylcellulose; 4, 6, 8, and 10, the enzyme plus $beta$ -1,3-xylan, $beta$ -1,4-xylan, curdlan, and carboxymethylcellulose, respectively.

	ACKNOWLEDGMENTS

We thank Shuichi Karita, Center for Molecular Biology and Genetics, Mie University, for performing sequencingprocedures.

	FOOTNOTES

^* Corresponding author. Mailing address: Faculty of Bioresources, Mie University, 1515 Kamihama, Tsu, Mie 514-8507,Japan.

REFERENCES

Top
Abstract
Text
References

1. Aoki, T., T. Araki, and M. Kitamikado. 1988. Purification and characterization of an endo- $beta$ -1,3-xylanase from Vibrio sp. Nippon Suisan Gakkaishi 54:277-281.

2. Araki, T., N. Inoue, and T. Morishita. 1998. Purification and characterization of $beta$ -1,3-xylanase from a marine bacterium, Alcaligenes sp. XY-234. J. Gen. Appl. Microbiol. 44:269-274.

3. Araki, T., S. Tani, K. Maeda, S. Hashikawa, H. Nakagawa, and T. Morishita. 1999. Purification and characterization of $beta$ -1,3-xylanase from a marine bacterium, Vibrio sp. XY-214. Biosci. Biotechnol. Biochem. 63:2017-2019[CrossRef][Medline].

4. Bailey, R. W., and E. J. Bourne. 1960. Colour reagents given by sugars and diphenylamineaniline spray reagents on paper chromatograms. J. Chromatogr. 4:206-213[CrossRef].

5. Beguin, P. 1983. Detection of cellulase activity in polyacrylamide gels using Congo red-stained agar replicas. Anal. Biochem. 131:333-336[CrossRef][Medline].

6. Biely, P. 1985. Microbial xylanolytic systems. Trends Biotechnol. 3:286-290[CrossRef].

7. Chen, W. P., M. Matsuo, and T. Yasui. 1986. Purification and some properties of $beta$ -1,3-xylanase from Aspergillus terreus A-07. Agric. Biol. Chem. 50:1183-1194.

8. Henrissat, B., and A. Bairoch. 1996. Updating the sequence-based classification of glycosyl hydrolases. Biochem. J. 316:695-696.

9. Iriki, Y., T. Suzuki, K. Nisizawa, and T. Miwa. 1960. Xylan of Siphonaceous green algae. Nature 187:82-83.

10. Laemmli, U. K. 1970. Cleavage of structural proteins during the assembly of the head of bacteriophage T4. Nature 227:680-685[CrossRef][Medline].

11. Lewin, B. 1997. Nucleic acid structure, p. 97-113. In B. Lewin (ed.), Genes VI. Oxford University Press, New York, N.Y.

12. Marchuk, D., M. Drumm, A. Saulino, and F. S. Collins. 1990. Construction of T-vectors, a rapid and general system for direct cloning of unmodified PCR products. Nucleic Acids Res. 19:1154[Free Full Text].

13. McDowell, R. H. 1967. Chemistry and enzymology of marine algal polysaccharides, p. 88-96. , 134-137. Academic Press, London, United Kingdom.

14. Mong, K. K. Y., L. U. L. Tan, and J. N. Saddler. 1988. Multiplicity of $beta$ -1,4-xylanase in microorganisms: functions and applications. Microbiol. Rev. 52:305-317[Free Full Text].

15. Ohmiya, K., K. Sakka, S. Karita, and T. Kimura. 1997. Structure of cellulase and their application. Biotechnol. Genet. Eng. Rev. 14:365-414[Medline].

16. Perlman, D., and H. O. Halvorson. 1983. A putative signal peptidase recognition site and sequence in eukaryotic and prokaryotic signal peptides. J. Mol. Biol. 167:391-409[CrossRef][Medline].

17. Senju, R., and S. Okimasu. 1950. Studies on chitin. Part I. On the glycolation of chitin and the chemical structure of glycol chitin. Nippon Nogeikagaku Kaishi 23:432-437. (In Japanese.)

18. Somogyi, M. 1952. Notes on sugar determination. J. Biol. Chem. 195:19-23[Free Full Text].

19. Timell, T. E. 1967. Recent progress in the chemistry of wood hemicelluloses. Wood Sci. Technol. 1:47-76.

20. von Heijne, G. 1986. A new method for predicting signal sequence cleavage sites. Nucleic Acids Res. 14:4683-4690[Abstract/Free Full Text].

21. Yamaura, I., T. Matumoto, M. Funatsu, and E. Murai. 1990. Purification and some properties of endo- $beta$ -1,3-xylanase from Pseudomonas sp. PT-5. Agric. Biol. Chem. 54:921-926[Medline].

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J. Bacteriol.	Microbiol. Mol. Biol. Rev.	Eukaryot. Cell	All ASM Journals

1.	Aoki, T., T. Araki, and M. Kitamikado. 1988. Purification and characterization of an endo- $beta$ -1,3-xylanase from Vibrio sp. Nippon Suisan Gakkaishi 54:277-281.
2.	Araki, T., N. Inoue, and T. Morishita. 1998. Purification and characterization of $beta$ -1,3-xylanase from a marine bacterium, Alcaligenes sp. XY-234. J. Gen. Appl. Microbiol. 44:269-274.
3.	Araki, T., S. Tani, K. Maeda, S. Hashikawa, H. Nakagawa, and T. Morishita. 1999. Purification and characterization of $beta$ -1,3-xylanase from a marine bacterium, Vibrio sp. XY-214. Biosci. Biotechnol. Biochem. 63:2017-2019[CrossRef][Medline].
4.	Bailey, R. W., and E. J. Bourne. 1960. Colour reagents given by sugars and diphenylamineaniline spray reagents on paper chromatograms. J. Chromatogr. 4:206-213[CrossRef].
5.	Beguin, P. 1983. Detection of cellulase activity in polyacrylamide gels using Congo red-stained agar replicas. Anal. Biochem. 131:333-336[CrossRef][Medline].
6.	Biely, P. 1985. Microbial xylanolytic systems. Trends Biotechnol. 3:286-290[CrossRef].
7.	Chen, W. P., M. Matsuo, and T. Yasui. 1986. Purification and some properties of $beta$ -1,3-xylanase from Aspergillus terreus A-07. Agric. Biol. Chem. 50:1183-1194.
8.	Henrissat, B., and A. Bairoch. 1996. Updating the sequence-based classification of glycosyl hydrolases. Biochem. J. 316:695-696.
9.	Iriki, Y., T. Suzuki, K. Nisizawa, and T. Miwa. 1960. Xylan of Siphonaceous green algae. Nature 187:82-83.
10.	Laemmli, U. K. 1970. Cleavage of structural proteins during the assembly of the head of bacteriophage T4. Nature 227:680-685[CrossRef][Medline].
11.	Lewin, B. 1997. Nucleic acid structure, p. 97-113. In B. Lewin (ed.), Genes VI. Oxford University Press, New York, N.Y.
12.	Marchuk, D., M. Drumm, A. Saulino, and F. S. Collins. 1990. Construction of T-vectors, a rapid and general system for direct cloning of unmodified PCR products. Nucleic Acids Res. 19:1154[Free Full Text].
13.	McDowell, R. H. 1967. Chemistry and enzymology of marine algal polysaccharides, p. 88-96. , 134-137. Academic Press, London, United Kingdom.
14.	Mong, K. K. Y., L. U. L. Tan, and J. N. Saddler. 1988. Multiplicity of $beta$ -1,4-xylanase in microorganisms: functions and applications. Microbiol. Rev. 52:305-317[Free Full Text].
15.	Ohmiya, K., K. Sakka, S. Karita, and T. Kimura. 1997. Structure of cellulase and their application. Biotechnol. Genet. Eng. Rev. 14:365-414[Medline].
16.	Perlman, D., and H. O. Halvorson. 1983. A putative signal peptidase recognition site and sequence in eukaryotic and prokaryotic signal peptides. J. Mol. Biol. 167:391-409[CrossRef][Medline].
17.	Senju, R., and S. Okimasu. 1950. Studies on chitin. Part I. On the glycolation of chitin and the chemical structure of glycol chitin. Nippon Nogeikagaku Kaishi 23:432-437. (In Japanese.)
18.	Somogyi, M. 1952. Notes on sugar determination. J. Biol. Chem. 195:19-23[Free Full Text].
19.	Timell, T. E. 1967. Recent progress in the chemistry of wood hemicelluloses. Wood Sci. Technol. 1:47-76.
20.	von Heijne, G. 1986. A new method for predicting signal sequence cleavage sites. Nucleic Acids Res. 14:4683-4690[Abstract/Free Full Text].
21.	Yamaura, I., T. Matumoto, M. Funatsu, and E. Murai. 1990. Purification and some properties of endo- $beta$ -1,3-xylanase from Pseudomonas sp. PT-5. Agric. Biol. Chem. 54:921-926[Medline].

Cloning, Sequencing, and Expression in Escherichia coli of the New Gene Encoding -1,3-Xylanase from a Marine Bacterium, Vibrio sp. Strain XY-214

Cloning, Sequencing, and Expression in Escherichia coli of the New Gene Encoding $beta$ -1,3-Xylanase from a Marine Bacterium, Vibrio sp. Strain XY-214