Method of predicting thermostable protein from mesophilic bacteria based on amino acid composition of thermophilic bacteria and its closely related methophilic bacteria, predicting program therefor and recording medium thereof

Information

  • Patent Application
  • 20050202409
  • Publication Number
    20050202409
  • Date Filed
    February 23, 2005
    19 years ago
  • Date Published
    September 15, 2005
    19 years ago
Abstract
The invention relates to a method of judging the thermostability of a protein, comprising the steps of calculating an analytical value specific to a test protein by a principal component analysis based on the amino acid composition of the protein calculated from the data of the amino acid sequence of the protein or the nucleotide sequence of the gene and comparing the analytical value with an analytical value of a protein which is retained by a thermostable organism and corresponds to the test protein, and further relates to a program for allowing a computer to execute processing for judging the thermostability of a protein by the method, and a computer readable recording medium having recorded the program thereon.
Description
BACKGROUND OF THE INVENTION

1. Field of the Invention


The present invention relates to a method of judging whether or not a protein has thermostability by focusing on a protein produced by an organism, and calculating a characteristic value related to thermostability from the data of the amino acid sequence or the nucleotide sequence of the protein. More particularly, the invention relates to a method of judging the thermostability of a protein, which judges whether or not a test protein has thermostability, comprising the steps of calculating an analytical value specific to the test protein by a principal component analysis based on the amino acid composition of the protein, and comparing the analytical value with an analytical value of a protein which is retained by a thermostable organism and corresponds to the test protein.


In addition, the invention relates to a program for judging whether or not the protein has thermostability by focusing on a protein produced by an organism, and calculating a characteristic value related to thermostability from the data of the amino acid sequence or the nucleotide sequence of the protein, and a recording medium having recorded the program thereon. More particularly, the invention relates to a program for allowing a computer to execute processing for judging the thermostability of a protein, which judges whether or not a test protein has thermostability by calculating an analytical value specific to the test protein by a principal component analysis based on the amino acid composition of the protein, and comparing the analytical value with an analytical value of a protein which is retained by a thermostable organism and corresponds to the test protein, and a computer readable recording medium having recorded the program thereon.


2. Background Art


Thermostable enzymes are widely used in the industrial world, research and development fields and the like as an enzyme that does not lose the enzymatic activity at a high temperature. Examples of the thermostable enzyme include, an enzyme used in an enzymatic reaction process for hydrolysis of a saccharide such as starch (see JP-T-10-506524 (the term “JP-T” as used herein means a published Japanese translation of a PCT patent application), and JP-A-2000-50870), an enzyme used in an enzymatic reaction in the disposal of food waste or in the production of a fertilizer from the food waste (see JP-A-2001-61474 and JP-A-2003-219864), an enzyme used in an enzymatic reaction in the production of a useful substance such as trehalose (see JP-A-08-336388 and JP-A-08-149980) and the like.


As described above, thermostable enzymes are very important in the industry. Recently, it has become important to develop a thermostable DNA polymerase to be used in the PCR method (see JP-B-04-67957), or in a replicative RNA-based amplification system (see JP-A-02-5864 and JP-A-02-500565), and a large number of thermostable DNA polymerases have been isolated mainly from thermophilic microorganisms. A DNA polymerase has become one of the important tools in genetic engineering techniques, and has become important as a tool not only for gene cloning or sequence determination, but also for detection or identification of a small amount of gene, namely, as an enzyme for gene amplification.


At present, thermostable DNA polymerases to be used mainly for these purposes are derived from the genus Thermus as Taq polymerase which is derived from T. aquaticus. The interest on the discovery of a novel polymerase with a more appropriate property and activity is growing, and as a DNA polymerase from other than the genus Thermus, for example, a method using a DNA polymerase from Anaerocellum thermophilum (see JP-T-2001-502169), a method using a DNA polymerase from a sulfur metabolism thermophilic archaebacterium Pyrococcus horikoshii (see JP-A-2000-41668) and the like have been reported.


In this way, the importance of thermostable enzymes is growing more and more, however, a search of such a thermostable enzyme often requires the steps of screening a bacterium producing a target enzyme from the natural world using thermophilic bacteria or thermostable bacteria as a target for screening, and confirming the thermostability of an enzyme produced by studying the culture conditions by performing a heat treatment one by one. Therefore, not only it required enormous time and effort, but also it depended on a coincidence in many cases. In addition, the subject of screening was limited to thermophilic bacteria, thermostable bacteria or mesophilic bacteria, and the thermophilic bacteria or thermostable bacteria was only limited species in light of numerous species of microorganisms, therefore the diversity of thermostable enzymes was limited.


Not only an accidental discovery is expected, but also the establishment of a systematic and saving method for searching a useful thermostable enzyme in industry was needed. Further, the development of a computer processable program, which is for conveniently executing the method was needed.


SUMMARY OF THE INVENTION

An object of the invention is to improve the conventional methods by which a thermostable enzyme search was performed through a trial and error process, and the invention provides a novel method which is a convenient method based on data such as the amino acid sequence or the nucleotide sequence of a protein and is capable of judging whether or not the protein has thermostability.


In addition, the invention provides a method capable of conveniently judging a wider variety of thermostable enzymes than ever by using resources of thermostable proteins such as useful enzymes as microorganisms for industry and thermostable enzymes to be used widely.


Further, an object of the invention is to improve the conventional methods by which a thermostable enzyme search was performed through a trial and error process, and the invention provides a computer program for judging whether or not a protein has thermostability by a convenient method based on data such as the amino acid sequence or the nucleotide sequence of the protein, data for the program and a recording medium of the program.


The present inventors carried out a principal component analysis by using the amino acid composition of a protein predicted in the genomes of 120 species of microorganisms whose complete genome sequences had been known until then, and calculated the principal component score of each protein based on the eigenvector of the second principal component (weighting factor of amino acid), and examined the correlation between the calculated value and the thermostability of the protein. As a result, they found out that there is an extremely strong correlation between the calculated value and the value of a protein which corresponds to the protein and is produced by a thermophilic bacterium. By utilizing this correlation, the inventors established a method capable of judging the thermostability of a protein, thus achieved the invention.


In addition, this method requires a large amount of data processing such as a search of a protein showing an orthologous relationship, calculation of a specific analytical value (vector value) by a principal component analysis of a test protein, and comparison with a known protein. Therefore, computerization of data processing such as calculation and search described above was needed. The inventors developed a program therefor and could complete the program.


In other words, the invention relates to a method of judging the thermostability of a protein, which judges whether or not a test protein has thermostability, comprising the steps of calculating an analytical value specific to the test protein by a principal component analysis based on the amino acid composition of the protein, and comparing the analytical value with an analytical value of a protein which is retained by a thermostable organism and corresponds to the test protein.


The invention provides a method of judging whether or not a protein has thermostability by using a specific analytical value obtained by a principal component analysis based on the amino acid composition of the protein, which is predicted from the data of the amino acid sequence or the nucleotide sequence of the protein, without performing a thermostability test of the protein.


The method of the invention can be programmed so as to be processed in a computer, and the invention provides a method capable of judging whether or not a protein has thermostability by inputting the data of the amino acid sequence or the nucleotide sequence of the protein into the program and allowing the computer to execute processing.


In addition, the invention relates to a program for allowing a computer to execute processing for judging the thermostability of a protein, which allows a computer to judge whether or not a test protein has thermostability, by calculating an analytical value specific to the test protein by a principal component analysis based on the amino acid composition of the protein, and comparing the analytical value with an analytical value of a protein which is retained by a thermostable organism and corresponds to the test protein.


Further, the invention relates to a program, which allows a computer to judge whether or not a test protein has thermostability by executing the steps of:

    • (1) inputting the amino acid sequence of the test protein,
    • (2) searching a known protein related to a protein corresponding to the test protein and produced by another species different from the one producing the test protein (hereinafter referred to as corresponding protein),
    • (3) calculating a specific analytical value by a principal component analysis based on the amino acid composition of the test protein,
    • (4) calculating the specific analytical value of the corresponding protein searched in the step (2) and the specific analytical value of the test protein calculated in the step (3), and calculating the difference between both values,
    • (5) judging whether or not the test protein is similar to the corresponding protein searched in the step (2) based on the difference calculated in the step (4), and
    • (6) displaying the corresponding protein searched in the step (2) and the result of judgment in the step (5),


      whereby the specific analytical value based on the amino acid composition of the test protein and the specific analytical value of the known corresponding protein are compared to judge whether or not the test protein has thermostability.


In addition, the invention relates to a computer readable recording medium having recorded thereon a program for allowing a computer to execute the program of the invention.




BRIEF DESCRIPTION OF THE DRAWINGS

The patent or application file contains at least one drawing executed in color. Copies of this patent or patent application publication with color drawing(s) will be provided by the U.S. Patent and Trademark Office upon request and payment of the necessary fee.



FIG. 1 is a phylogenetic tree created by the neighbor-joining method based on 16S rDNA sequences of Bacillus-related species used in a method of the invention as an example.



FIG. 2 is a colored graph showing the results of analyzing the amino acid compositions of proteins retained by 120 species of microorganisms whose complete genome sequences have been known so far by a principal component analysis (PCA). The first principle component (PC1) was defined as the GC content and the second principal component (PC2) was defined as the upper limit temperature for growth.



FIG. 3 shows a correlation chart based on the value of the “principal component score” of each protein for Geobacillus stearothermophilus (GS), which has substantially the same upper limit temperature for growth as that of thermophilic Geobacillus kaustophilus (GK). In FIG. 3, the horizontal axis represents the values of the “principal component score” of GK, and the vertical axis represents the values of the “principal component score” of GS.



FIGS. 4A to 4D are graphs showing the correlations between thermophilic G. kaustophilus (GK) and mesophilic bacteria, Bacillus cereus (BC) (FIG. 4A), Bacillus halodurans (BH) (FIG. 4B), Bacillus subtilis (BS) (FIG. 4C) and Oceanobacillus iheyensis (OI) (FIG. 4D), respectively. The horizontal axes of the respective graphs represent the values of the “principal component score” of GK, and the vertical axes of the respective graphs represent the values of the “principal component score” of each mesophilic bacterium, respectively.



FIG. 5 is a graph summarizing the relationship between the upper limit temperatures for growth of the respective microorganisms, GK (closed square ▪), BC (open triangle Δ), BH (closed circle ●), BS (open circle ◯) and OI (open square □) and the ratio of the proteins among the 965 proteins in the case where the difference in the values of the “principal component scores” between GK and each of the other microorganisms varies. In FIG. 5, the horizontal axis represents the temperature and the vertical axis represents the ratio (%). On the horizontal axis, the upper limit temperatures for growth of the respective microorganisms are plotted. On the vertical axis, with regard to the upper line (indicated in green in the original figure), the ratios (%), relative to all the 965 proteins, of the number of proteins in the case where the difference in the values of the “principal component scores” between GK and each of the other microorganisms is greater than −0.015 are plotted for each of the microorganisms, with regard to the line in the middle (indicated in blue in the original figure), the ratios (%) of the number of proteins in the case where the difference is greater than −0.010 are plotted for each of the microorganisms, and with regard to the lower line (indicated in red in the original figure), the ratios (%) of the number of proteins in the case where the difference is greater than −0.005 are plotted for each of the microorganisms.



FIGS. 6A and 6B are photographs substituted for a drawing, which show the results of examining the native-PAGE patterns after separating the proteins of the respective microorganisms, GK, BC, BH, BS and OI. FIG. 6A shows the bands of all the proteins, and FIG. 6B shows the bands of proteins with an esterase activity of each microorganism. GK, BC, BH, BS and OI in the respective figures represent the respective microorganisms, and with regard to the respective lanes 1 to 3 for each of the microorganisms, lane 1 corresponds to a sample without heat treatment, lane 2 corresponds to a sample with heat treatment at 60° C. for 10 minutes, and lane 3 corresponds to a sample with heat treatment at 70° C. for 10 minutes.



FIGS. 7A and 7B are photographs substituted for a drawing, which show the results of examining the native-PAGE patterns after separating Hag and GroES proteins of the respective microorganisms, GK, BC, BH, BS and OI. FIG. 7A shows the native-PAGE patterns of Hag, and FIG. 7B shows the native-PAGE patterns of GroES. GK, BC, BH, BS and OI in the respective figures represent each of the microorganisms, and with regard to the respective lanes 1 to 3 for each of the microorganisms, lane 1 corresponds to a sample without heat treatment, lane 2 corresponds to a sample with heat treatment at 60° C. for 10 minutes, and lane 3 corresponds to a sample with heat treatment at 70° C. for 10 minutes.



FIG. 8 is a flowchart showing processing from the user viewpoint in the program of the invention.



FIG. 9 is a flowchart showing input processing from the server viewpoint in the program of the invention.



FIG. 10, consisting of FIGS. 10A through 10O, is a color version of Table 1 showing the prediction of thermostability of proteins possessing one-to one correspondence among 5 species of Bacillus.




DETAILED DESCRIPTION OF THE INVENTION

The method of the invention of judging whether or not a test protein has thermostability will be explained.


It is known that there is a correlation between the amino acid compositions of all the proteins deduced from the genome sequence of a microorganism whose complete nucleotide sequences have been determined and the growth temperature of the microorganism. In particular, it is known that the correlation is significantly observed in hyper thermophilic archaebacteria (Archaea) that grows at over 80° C. and in some bacteria. However, almost all the hyper thermophilic bacteria whose complete genome sequences have been determined belongs to Archaea, and detail investigation whether the correlation is specific to Archaea or is a characteristic of thermophilic bacteria has not been carried out. In a similar way, with regard to some thermophilic bacteria whose genome sequence determination has been completed, there are no mesophilic or non-thermostable bacteria closely related to the thermophilic bacteria, or if there is, there is no genome sequence information thereof. Therefore, it was difficult to accurately determine whether the characteristic of the amino acid composition observed in the thermophilic bacteria is indeed a characteristic specific to thermophilic bacteria or it simply reflects a specificity of the species.


In order to accurately determine such a correlation, the inventors decided to investigate the correlation between genome sequence information and thermostability by focusing on Bacillus-related species in which thermophilic bacteria whose upper limit temperature for growth is approximately 70° C. and mesophilic bacteria whose upper limit temperature for growth varies exist in the same genus and a closely related genus. Among the Bacillus-related species, the complete genome sequences of 4 species of mesophilic bacteria, B. subtilis, B. halodurans, O. iheyensis and B. cereus have been revealed, however, the complete genome information of thermophilic Bacillus-related species has not been analyzed.


Therefore, it was decided that the genome of G. kaustophilus HTA426 (hereinafter abbreviated as GK), which is one species of thermophilic G. kaustophilus would be analyzed. This microorganism was obtained from the deep-sea of Mariana Trench. Its upper limit temperature for growth is 74° C.


A phylogenetic tree created by the neighbor-joining method based on 16S rDNA sequences of these Bacillus-related species is shown in FIG. 1. The bar in the lower left in FIG. 1 indicates 0.01 Knuc unit. The part indicated with the lower line (indicated in red in the original figure) indicates that they are thermophilic bacteria. The 5 species of microorganisms, from the upper-side, B. halodurans C-125 (hereinafter abbreviated as BH), B. subtilis 168 (hereinafter abbreviated as BS), B. cereus ATCC14579 (hereinafter abbreviated as BC), O. iheyensis HTE831 (hereinafter abbreviated as OI) and G. kaustophilus HTA426 (hereinafter abbreviated as GK) used in the following analysis are marked with asterisks at the upper right thereof.


First, the inventors determined the complete nucleotide sequence of the genome sequence of thermophilic G. kaustophilus. Next, they analyzed the amino acid compositions of the proteins retained by the 5 species of microorganisms including the G. kaustophilus (GK) and 120 species of microorganisms whose complete genome sequences have been known so far by a principal component analysis (PCA). As a result, as is conventionally known, it was observed that the PC1 shows a strong correlation with the GC content and the PC2 shows a strong correlation with the upper limit temperature for growth in whole.


This result is shown in FIG. 2. The original figure of FIG. 2 is a colored graph. The horizontal axis represents the analytical values of the GC content (PC1), and the vertical axis represents the analytical values of the upper limit temperature for growth (PC2). The PCA performed here was in accordance with a usual method in statistics. The red square (black in the black and white figure) indicates thermophilic bacteria, the blue (black in the black and white figure) indicates Gram-positive bacteria with low GC content, and the green (slightly gray in the black and white figure) indicates Gram-positive bacteria with high GC content. The line at 0.0152 of the PC2 score indicates the boundary between thermophilic bacteria (upper side) and mesophilic bacteria (lower side).


In addition, even if it is limited to the Bacillus-related species, a correlation between the second principal component score and the upper limit temperature for growth was observed. However, the result was obtained by using the average amino acid composition of the entire bacteria, and when considering the individual proteins, they were widely scattered; therefore, the correlation was not so clear.


Accordingly, the inventors first calculated the thermostability index of each protein for the 5 species of microorganisms related to the genus Bacillus used in the analysis by multiplying an eigenvector corresponding to the second principal component by an amino acid composition as a weighting factor.


The PCA based on the amino acid compositions used here was carried out by obtaining the genome data of 119 species of microorganisms from the database at NCBI, and using the protein sequences identified in the genomes of 120 species including the obtained genomes of 119 species and the genome of G. kaustophilus HTA426, which had been determined in the invention. From these sequences, a sequence with a sequence length of less than 50 amino acids was excluded, further a protein which had been predicted to contain 2 or more transmembrane domains by the PSORT program was also excluded. By using the sequences of the remaining proteins, an average amino acid composition was calculated on a species basis, a matrix in which each row and column corresponds to the species and an amino acid, respectively, was input, and a principal component analysis was performed using the princomp function in the R statistical analysis package.


Subsequently, based on the results, the differences between the principal component score of a corresponding protein of thermophilic G. kaustophilus and those of the 4 species of mesophilic bacteria were calculated. This grouping was performed based on an orthologous relationship deduced from a homology search result, and analysis was performed by using a protein having one-to-one correspondence as a target (Kreil D. P. and Ouzounis, C. A. (2001), Identification of thermophilic species by the amino acid compositions deduced from their genome. Nucleic acids Res. 29, 1608-1615).


The selected 965 proteins are a protein which does not contain 2 or more transmembrane domains, and 965 proteins which are common in the 5 species were extracted from the genome server of G. stearothermophilus (hereinafter abbreviated as GS) which has substantially the same upper limit temperature for growth as GK. The judgment whether or not a protein contains 2 or more transmembrane domains was performed by the PSORT program (Nakai, K. & Horton, P., PSORT: Trends Biochem. Sci., 24, 34-36 (1999)).


The values of the calculated “principal component score” from the result are shown in Table 1, shown in color in FIGS. 10A-10O. Each of the columns of the tables corresponds to, from the left, “GK ID” indicating an identification signal based on GK, “category” indicating the classification of each protein, “annotation” indicating the name or the like of each protein, and in the right side, the ID signal of each of the 5 species of microorganisms and the value of the “principal component score”, being placed in the order of GK, BC, BH, BS and OI from the left. With regard to the color of the identification signal of each microorganism, (see FIGS. 10A-10O), red indicates the case in which the difference in the “principal component scores” of corresponding proteins of GK and each of the other species (difference=(each score for each microorganism)−(each score for GK)) is −0.005 or lower, blue indicates the case in which the difference is −0.010 or lower, green indicates the case in which the difference is −0.015 or lower, and no color indicates the case in which the difference is greater than −0.015.
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As is clear from the results, it has been demonstrated that even if a clear correlation cannot be observed in all the microorganisms, by comparing individual proteins corresponding to each other, there is a case where a clear correlation exists. In order to clarify it more clearly, the correlation between GK and each of the microorganisms is shown in a graph.


In order to make a graph, an orthologous grouping with G. stearothermophilus (GS), which has substantially the same upper limit temperature for growth as GK was performed as follows. A draft genome sequence of GS was obtained from the FTP site at the University of Oklahoma. By using each translated sequence of GK as a query, a similar sequence was searched against these contig sequences with the TBLASTN program, and the resulting sequence with the best score was taken as an orthologue when it covered 70% or more of the length of the query sequence with 70% or more identity. Next, with regard to GK and GS, a correlation chart based on the value of the “principal component score” of each protein is shown in FIG. 3. In FIG. 3, the horizontal axis represents the values of the “principal component score” of GK, and the vertical axis represents the values of the “principal component score” of GS. The solid line in the graph indicates that both values are the same, and the dashed lines indicate the range within ±0.01 from the solid line. In this way, it is found that in the case of comparing proteins among thermophilic bacteria, the values of the “principal component scores” of the respective proteins have an extremely strong correlation. Similarly, graphs showing correlations of GK with mesophilic bacteria, BC, BH, BS and OI are shown in FIGS. 4A to 4D, respectively. FIG. 4A shows the correlation of GK with BC, FIG. 4B shows the correlation of GK with BH, FIG. 4C shows the correlation of GK with BS and FIG. 4D shows the correlation of GK with OI. The horizontal axes of the respective graphs represent the values of the “principal component score” for GK, and the vertical axes of the respective graphs represent the values of the “principal component score” for each mesophilic bacterium, respectively. From these graphs, it is found that with regard to mesophilic bacteria, some proteins show a good correlation with those of GK, but some proteins show completely different values depending on the types of the proteins.


With regard to the correlation of GK with GS, almost all the proteins show a strong correlation, however, comparison of GK with the mesophilic bacteria demonstrates that some proteins show almost no correlation. It might be considered that this is because the proteins do not have thermostability. On the contrary, mesophilic bacteria lack thermostability as a whole, however, it might be considered that not all the proteins produced by the microorganisms lack thermostability, but what lacks thermostability is some of the proteins. Suppose a protein that lacked thermostability was essential to life, even if all the other proteins have thermostability, the microorganism would no longer have thermostability as a whole organism.


This is a new finding in the invention of the inventors. In other words, conventionally, in the case of searching a thermostable protein, the search was performed by screening a thermostable microorganism. This is because a thermostable organism has a thermostable protein, otherwise, it cannot maintain its life under a high temperature condition. However, it is not always the case where all the proteins produced by a mesophilic bacterium must lack thermostability. It is not always the case where, even if a mesophilic bacterium produces a thermostable protein, a problem on maintaining its life will occur. It is quite considerable that the reason why a mesophilic bacterium is not thermostable is that not all the proteins lack thermostability, but a protein essential to life lost thermostability.


The results shown in Table 1 and FIG. 4 indicate the possibility that even a mesophilic bacterium produces a similar thermostable protein, which is produced by a thermophilic bacterium.


These results are summarized based on the correlation with the upper limit temperatures for growth of the respective microorganisms and shown in FIG. 5. In FIG. 5, the horizontal axis represents the temperature and the vertical axis represents the ratio (%). In the graph, the closed square (▪) represents GK, the closed circle (●) represents BH, the open circle (◯) represents BS, the open triangle (Δ) represents BC and the open square (□) represents OI. On the horizontal axis, the upper limit temperatures for growth of the respective microorganisms are plotted. On the vertical axis, with regard to the upper line (indicated in green in the original figure), the ratios (%), relative to all the 965 proteins, of the number of proteins in the case where the difference in the values of the “principal component scores” between GK and each of the other microorganisms is greater than −0.015 are plotted for each of the microorganisms, with regard to the line in the middle (indicated in blue in the original figure), the ratios (%) of the number of proteins in the case where the difference is greater than −0.010 are plotted for each of the microorganisms, and with regard to the lower line (indicated in red in the original figure), the ratios (%) of the number of proteins in the case where the difference is greater than −0.005 are plotted for each of the microorganisms. A protein in the case where the difference in the values of the “principal component scores” is greater than −0.015 (i.e., −0.015 or higher, the absolute value becomes small, however, it is a minus number, therefore, it becomes large, hereinafter the same as above) is defined as a thermostable protein, and the number of proteins of these bacteria, BC, BH, BS and OI and the ratio are summarized and shown in Table 2.

TABLE 2Summary of prediction of thermostable proteins from bacteria belonging tomesophilic Bacillus species based on the principal component analysisBCBHBSBSOIprediction(number)BC (%)(number)BH (%)(number)(%)(number)OI (%)15916.520220.926927.939140.5+959.8838.610811.211011.4++12813.3145151351412012.4+++58360.453555.445346.934435.6++, +++71173.768070.568860.946448.1+, ++, +++80683.576379.169672.157459.5


The Table 2 summarizes the results of prediction of thermostable proteins from bacteria belonging to mesophilic Bacillus species based on the principal component analysis. In Table 2, “−” indicates the case where the difference in PC2 values of the proteins of each microorganism and GK is lower than −0.015, thereby being judged lack of thermostability, and “+”, “++”, “30 ++” indicate the cases where the difference is greater than −0.015, −0.01 and −0.005, respectively, thereby being judged presence of thermostability. In Table 2, “++, +++” corresponds to the sum of the numbers of “++” and “+++”, and “+, ++, +++” corresponds to the sum of the numbers of “+”, “++” and “+++”. Table 2 summarizes the results of analysis based on 965 orthologues having one-to-one correspondence among the 5 Bacillus-related species.


As a result, as shown in Table 2, the ratios of the proteins predicted to be thermostable among the 965 proteins are 83.5% for BC, 79.1% for BH, 72.1% for BS, and 59.5% for OI, respectively. In the graph of FIG. 5, BC (Δ) shows somewhat abnormal values, however, it is found that the other three species show similar tendencies. In other words, it is demonstrated that the more proteins with a value of “principal component score” equal to that of a protein produced by a thermophilic bacterium produces a microorganism, the higher becomes the upper limit temperature for growth of the microorganism. For example, with regard to OI that produces the fewest proteins with a value of “principal component score” equal to that of a protein produced by a thermophilic bacterium, its upper limit temperature for growth is the lowest among these microorganisms. Incidentally, BC (Δ) has the largest amount of the same types of proteins among the 4 mesophilic bacteria, however, it is found that its upper limit temperature for growth is abnormally low. It is considered that this is because a protein essential to life retained by BC happened to lose thermostability.


Subsequently, in order to verify the foregoing results, proteins were isolated from these microorganisms, and subjected to the following treatments: (1) no heat treatment, (2) heat treatment at 60° C. for 10 minutes, or (3) heat treatment at 70° C. for 10 minutes, respectively, and the native-PAGE patterns were examined. The results are shown in the photographs substituted for a drawing in FIGS. 6A and 6B. FIG. 6A shows the native-PAGE patterns of all the proteins stained with Coomassie Brilliant Blue. From the result, with regard to GK, a thermophilic bacterium, almost all the protein bands could be confirmed even after the heat treatment (lanes 2 and 3), however, it is found that with regard to the other 4 species of mesophilic bacteria, a lot of protein bands were lost by the heat treatment. What is important here is that not all the protein bands were lost. It is found that some protein bands remained without being lost after the heat treatment. The results demonstrate that not all the proteins produced even by a mesophilic bacterium are not thermostable.



FIG. 6B shows the results of detecting the bands of proteins with an esterase (EC 3.1.1.1) activity by active staining after all the proteins of each microorganism were separated by native PAGE in the same manner as in FIG. 6A. BC, BH, BS, GK and OI in the respective figures represent the respective microorganisms. With regard to the respective lanes 1 to 3 for each of the microorganisms, lane 1 corresponds to a sample without heat treatment, lane 2 corresponds to a sample with heat treatment at 60° C. for 10 minutes, and lane 3 corresponds to a sample with heat treatment at 70° C. for 10 minutes. In the case of OI in FIG. 6B with regard to esterase, the bands were lost by the heat treatment at 60° C. (lane 2). In addition, in the case of BC, the main band which had been most intensively stained in the case where heat treatment had not been applied was lost by the heat treatment. However, in the case of BS, the bands were not lost by the heat treatment, and in the case of BH, the bands, although they were faint, remained without being lost even by the heat treatment at 60° C.


In addition, with regard to GroES that is one of the proteins essential to growth for B. subtilis, and Hag (Flagellin) that is one of the representative proteins retained commonly by Bacillus-related species, the genes encoding these proteins were amplified by PCR from the respective microorganisms, and by using the cloned genes with E. coli, the same verification of thermostability as above was carried out. The cloned and purified proteins were subjected to the following treatments: (1) no heat treatment, (2) heat treatment at 60° C. for 10 minutes, and (3) heat treatment at 70° C. for 10 minutes, respectively, and then the native-PAGE patterns were examined. The results are shown in the photographs substituted for a drawing in FIGS. 7A and 7B. FIG. 7A shows the native-PAGE patterns of Hag, and FIG. 7B shows the native-PAGE patterns of GroES, which were obtained by separating the proteins with native PAGE and staining them with Coomassie Brilliant Blue. BC, BH, BS, GK and OI in the respective figures represent the respective microorganisms, and with regard to the respective lanes 1 to 3 for each of the microorganisms, lane 1 corresponds to a sample without heat treatment, lane 2 corresponds to a sample with heat treatment at 60° C. for 10 minutes, and lane 3 corresponds to a sample with heat treatment at 70° C. for 10 minutes.


Another problem is what types of proteins are thermostable. It was found that, in the case of esterase, it is difficult to specify which band corresponds to esterase specifically because plural proteins might be stained by a staining method, therefore, the inventors decided to focus on the proteins, Hag and GroES. The results of verification of Hag and GroES of each microorganism are shown in FIGS. 7A and 7B, respectively. These proteins have the identification signal of GK, GK3131 (Hag) and GK0248 (GroES) described in the Tables above.


The values of the principal component scores of these proteins for each microorganism are as follows: with regard to Hag, (GK, −0.0513; BC, −0.0622; BH, −0.0567; BS, −0.0578; OI, −0.0528) (see Table 1), with regard to GroES, (GK, 0.1018; BC, 0.0826; BH, 0.1012; BS, 0.0940; OI, 0.0988) (see Table 1). These are summarized and shown in the following Table 3.

TABLE 3GKBCBHBSOIHag (GK3131)−0.0513−0.0622−0.0567−0.0578−0.0528difference with GK0.01090.00540.00650.0015GroES (GK0248)0.10180.08260.10120.09400.0988difference with GK0.01920.00060.00780.0030


With regard to Hag protein, the bands were maintained even by the heat treatment at 70° C. in substantially the same manner as in the case of no heat treatment for all microorganisms except for BC. With regard to GroES protein, only faint bands were confirmed by the heat treatment at 60° C. or higher for BC and BS, therefore, it is considered that the proteins were decomposed by the heat treatment. For the other microorganisms, BH, OI and GK, the bands were maintained in the same manner as in the case of no heat treatment. These results demonstrated that in mesophilic bacteria, some proteins have thermostability, and some proteins do not depending on their types.


Subsequently, the protein bands remaining without being lost after the heat treatment at 70° C. for 10 minutes shown in FIG. 6A were cut out from the gel in the order from the upper part, and identification of the proteins contained in each band was performed using LC/MS/MS. The results are shown in Tables 4 to 7.

TABLE 4List of thermostable proteins from Bacillus subtilis confirmed experimentally and its comparison with computationalprediction of the thermostabilityDifference in scoresof principalCorrespondingNumber ofComponent analysisGene namegene nameResult ofamino aids ofbetweenof BSProduct nameof GKPredictionthe productgk and bsnadENH3-dependent NAD+ synthetase (sporulation proteinGK2596272−0.0340out B) (general stress protein 38)yjcGhypothetical protein (yjcG)GK0864171−0.0200codYtranscriptional regulatorGK1215259−0.0270ymfGprocessing proteaseGK1287240−0.0420deoDpurine nucleoside phosphorylaseGK1580233−0.0190ypfDribosomal protein S1 homolog (jofD)GK2225382−0.0155efpelongation factor PGK2410185−0.0152yqhTXaa-Pro dipeptidaseGK2411353−0.0233etfBelectron transfer flavoprotein (beta subunit)GK2687257−0.0205ytdIhypothetical proteinGK2792267−0.0243tyrStyrosyl-tRNA synthetaseGK2803422−0.0156yugJNADH-dependent butanol dehydrogenaseGK2925387−0.0290enoenolaseGK3054430−0.0184hutIimidazolone-5-propionate hydrolaseGK1368421−0.0296clpCclass III stress response-related ATPaseGK0078+810−0.0132rplBribosomal protein L2GK0109+277−0.0106acoBacetoin dehydrogenase E1 component (TPP-dependentGK0711+342−0.0112beta subunit)pycApyruvate carboxylaseGK1079+1148−0.0147ftsZcell-division initiation proteinGK1125+382−0.0113sucDsuccinyl-CoA synthetase (alpha subunit)GK1209+300−0.0111pnpApolynucleotide phosphorylase (PNPase)GK1269+705−0.0124hbsnon-specific DNA-binding protein HBsuGK2215+92−0.0118drmphosphodeoxyribomutaseGK2314+394−0.0144yqjMNADH-dependent flavin oxidoreductaseGK2332+338−0.0101zwfglucose-6-phosphate 1-dehydrogenase (pentoseGK2334+489−0.0147bcdleucine dehydrogenaseGK2381+364−0.0109aspSaspartyl-tRNA synthetaseGK2572+592−0.0108queAS-adenosylmethionine tRNA ribosyltransferaseGK2588+342−0.0132yufOABC transporterGK1284+510−0.0137yurXhypothetical proteinGK2994+437−0.0118citGfumarate hydrataseGK0250+462−0.0114hprKhypothetical proteinGK3082+310−0.0133nfrANADPH-flavin oxidoreductase(ipa-43d)GK1652+249−0.0141mmsAmethylmalonate-semialdehyde dehydrogenaseGK1887+487−0.0104metSmethionyl-tRNA synthetaseGK0031++664−0.0052rplLribosomal protein L12 (BL9)GK0096++123−0.0086rpoARNA polymerase (alpha subunit)GK0133++314−0.0064ylbAhypothetical protein (ylbA)GK1089++120−0.0081proSprolyl-tRNA synthetaseGK1257++564−0.0052infBtranslation initiation factor IF-2GK1263++716−0.0065citBaconitate hydrataseGK1347++909−0.0075odhA2-oxoglutarate dehydrogenase (E1 subunit)GK1023++941−0.0099ribHriboflavin synthase (beta subunit)GK2294++154−0.0066yqkFhypothetical proteinsGK2321++306−0.0060hemLglutamate-1-semialdehyde 2,1-aminotransferaseGK2642++430−0.0081pykpyruvate kinaseGK2739++585−0.0074hagflagellin proteinGK3131++304−0.0063rocFarginaseGK0149++296−0.0059guaBinositol-monophosphate dehydrogenaseGK0009+++488−0.0003hprThypoxanthine-guanine phosphoribosyltransferaseGK0061+++1800.0098gltXglutamyl-tRNA synthetaseGK0083+++4830.0061rpoBRNA polymerase (beta subunit)GK0098+++1193−0.0021fusAelongation factor GGK0103+++6920.0066tufAelongation factor TuGK0104+++3960.0041ybbTphosphoglucomutase (glycolysis)GK0154+++4480.0033groELclass I heat-shock protein (molecular chaperonin)GK0249+++544−0.0003guaAGMP synthetaseGK0254+++5130.0048gatBglutamyl-tRNA(Gln) amidotransferaseGK0283+++4760.0071glpKglycerol kinaseGK1360+++4960.0000yhxBphosphomannomutaseGK0570+++5650.0067datD-alanine aminotransferaseGK0672+++282−0.0031yheAhypothetical protein (yheA)GK0640+++1170.0429serCphosphoserine aminotransferaseGK0649+++359−0.0041argFornithine carbamoyltransferaseGK0796+++319−0.0015yjbGoligoendopeptidaseGK0822+++609−0.0038ykrSinitiation factor eIF-2B (alpha subunit)GK0949+++353−0.0035ptsIphosphotransferase system (PTS) enzyme IGK0996+++5700.0090ampSaminopeptidaseGK2140+++4100.0171pdhBpyruvate dehydrogenase (E1 beta subunit)GK1059+++325−0.0034dihydrolipoamide dehydrogenase E3 subunit of bothpdhDpyruvate dehydrogenase and 2-oxoglutarateGK1061+++4700.0072dehydrogenase complexessucCsuccinyl-CoA synthetase (beta chain)GK1208+++385−0.0030tsfelongation factor TsGK1250+++293−0.0036nusAtranscription termination (nusA)GK1260+++3710.0195cinAcompetence-damage inducible proteinGK1294+++4160.0143glnAglutamine synthetaseGK1327+++4440.0074odhB2-oxoglutarate dehydrogenase complexGK1024+++4170.0093asnSasparaginyl-tRNA synthetaseGK2171+++4300.0035aspBaspartate aminotransferaseGK2172+++3930.0069panCpantothenate synthetaseGK2178+++2860.0086ndknucleoside diphosphate kinaseGK2209+++1490.0069lysAdiaminopimelate decarboxylase (DAP decarboxylase)GK2300+++439−0.0040yqjI6-phosphogluconate dehydrogenase (pentoseGK2344+++469−0.0042sodAsuperoxide dismutaseGK2457+++2020.0028sigARNA polymerase major sigma-43 factor (sigma-A)GK2482+++371−0.0007dnaKclass I heat-shock protein (chaperonin)GK2504+++6110.0084yrbEopine catabolismGK1897+++3410.0102valSvalyl-tRNA synthetaseGK2638+++880−0.0020hemBdelta-aminolevulinic acid dehydrataseGK2643+++324−0.0031tigtrigger factor (prolyl isomerase)GK2653+++4240.0062mdhmalate dehydrogenaseGK2734+++3120.0003icdisocitrate dehydrogenaseGK2735+++423−0.0047citZcitrate synthase IIGK2736+++372−0.0039tpxthiol peroxidaseGK2787+++1670.0171acsAacetyl-CoA synthetaseGK2806+++5720.0007pckAphosphoenolpyruvate carboxykinaseGK2850+++5270.0113pgiglucose-6-phosphate isomeraseGK2924+++451−0.0047aldL-alanine dehydrogenaseGK3448+++378−0.0037yumCthioredoxin reductaseGK2954+++3320.0113yurUhypothetical proteinGK2991+++4650.0069yurYABC transporter (ATP-binding protein)GK2995+++261−0.0007yusJbutyryl-CoA dehydrogenaseGK3006+++594−0.0008pgmphosphoglycerate mutaseGK3055+++511−0.0048yvbYhypothetical proteinGK0393+++2400.0240clpPATP-dependent Clp protease proteolytic subunit (classGK3062+++1970.0157III heat-shock protein)rbsKribokinaseGK3230+++2930.0075atpDATP synthase (subunit beta)GK3358+++473−0.0048atpAATP synthase alpha chainGK3360+++502−0.0043glyAserine hydroxymethyltransferaseGK3369+++4150.0094ywjHtransaldolase (pentose phosphate)GK3385+++212−0.0014fbaAfructose-1,6-bisphosphate aldolaseGK3386+++285−0.0031ptaphosphotransacetylaseGK3415+++3230.0000fbaBmyo-inositol catabolism (yxdH)GK1892+++2780.0033iolDalternate gene name: yxdC˜myo-inositol catabolismGK1888+++3250.0157ahpCalkyl hydroperoxide reductase (small subunit)GK2575+++1870.0115ahpFalkyl hydroperoxide reductase (large subunit) andGK2574+++5090.0085NADH dehydrogenasepurAadenylosuccinate synthetaseGK3475+++430−0.0049yyaFhypothetical proteinGK3483+++366−0.0049
Difference in scores of principal component analysis between gk and bs

−: <−0.015 to be judjed as lack of thermostability

+: >−0.015 to be judged to have thermostability

++: >−0.010 to be judged to have thermostability

+++: >− to be judged to have thermostability









TABLE 5










List of thermostable proteins from Bacillus halodurans confirmed experimentally and its comparison


with computational prediction of the thermostability














Corresponding

Number of amino
Difference in scores of


Gene name

gene name of
Result of
aids of the
principal component analysis


of BH
Product name
GK
Prediction
product
between gk and bh















BH3347
polyribonucleotide
GK2927

138
−0.0335



nucleotidvltransferase (general stress


BH3556
enolase (2-phosphoglycerate
GK3054

429
−0.0160


BH2469
succinyl-CoA synthetase (alpha subunit)
GK1209
+
302
−0.0148


BH3053
trigger factor (prolyl isomerase)
GK2653
+
431
−0.0112


BH3099
electron transfer flavoprotein (alpha
GK2686
+
325
−0.0133


BH3100
electron transfer flavoprotein (beta
GK2687
+
256
−0.0134


BH0906
catalase
GK1710
++
735
−0.0098


BH1309
non-specific DNA-binding protein II
GK2215
++
90
−0.0100


BH1409
superoxide dismutase
GK2457
++
202
−0.0088


BH1530
phosphopentomutase
GK2314
++
393
−0.0063


BH3059
ketol-acid reductoisomerase
GK2659
++
340
−0.0070


BH3257
endo-1,4-beta-glucanase
GK2820
++
357
−0.0051


BH3560
glyceraldehyde-3-phosphate
GK3058
++
335
−0.0092


BH0020
inositol-monophosphate dehydrogenase
GK0009
+++
485
0.0005


BH0063
translation initiation inhibitor
GK0041
+++
124
0.0202


BH0122
50S ribosomal protein L7/L12
GK0096
+++
121
0.0005


BH0132
translation elongation factor Tu (EF-
GK0104
+++
396
0.0029


BH0562
class I heat-shock protein (chaperonin)
GK0249
+++
544
−0.0025


BH0613
endo-1,4-beta-glucanase
GK1868
+++
807
0.0033


BH1018
stress-and starvation-induced gene
GK2861
+++
146
−0.0005



controlled by sigma-B


BH1149
unknown conserved protein
GK0640
+++
116
−0.0008


BH1177
protein secretion (post-translocation
GK0656
+++
333
0.0030


BH1345
heat-shock protein (activation of DnaK)
GK2505
+++
194
0.0185


BH1346
class I heat-shock protein (chaperonin)
GK2504
+++
614
−0.0022


BH1385
ATP-dependent RNA helicase
GK2475
+++
438
−0.0028


BH1515
PTS system, glucose-specific enzyme II
GK3446
+++
173
0.0004


BH1604
inorganic pyrophosphatase
GK2246
+++
163
0.0049


BH1636
30S ribosomal protein S1
GK2225
+++
383
−0.0045


BH1654
nucleoside diphosphate kinase
GK2209
+++
147
0.0213


BH2360
glutamine synthetase
GK1327
+++
449
0.0031


BH2426
elongation factor Ts
GK1250
+++
293
0.0235


BH2470
succinyl-CoA synthetase (beta subunit)
GK1208
+++
386
0.0008


BH2665
2-cys peroxiredoxin
GK2575
+++
183
0.0110


BH2800
Xaa-Pro dipeptidase
GK2411
+++
355
0.0006


BH3558
triosephosphate isomerase
GK3056
+++
251
0.0162


BH3616
flagellin
GK3131
+++
272
−0.0045


BH3786
fructose-1,6-bisphosphate aldolase
GK3386
+++
287
−0.0021


BH3793
DNA-directed RNA polymerase delta
GK3390
+++
164
0.0264







Difference in scores of principal component analysis between gk and bh





−: <−0.015 to be judjed as lack of thermostability





+: >−0.015 to be judged to have thermostability





++: >−0.010 to be judged to have thermostability





+++: >−0.005 to be judged to have thermostability














TABLE 6










List of thermostable proteins from Oceanobacillus iheyensis confirmed experimentally and


its comparison with computational prediction of the thermostability














Corresponding


Difference in scores of


Gene name of

gene name of
Result of
Number of amino
principal component analysis


OB
Product name
GK
Prediction
aids of the product
between gk and oi















OB1216
thimet oligopeptidase
GK0822

602
−0.0179


OB2345
purine nucleoside phosphorylase
GK1580

235
−0.0249


OB1528
chromosome segregation SMC protein
GK1193

1188
−0.0166


OB2002
transcriptional elongation factor
GK2547

158
−0.0169


OB1800
30S ribosomal protein S1
GK2225

376
−0.0281


OB1969
heat shock protein
GK2505

190
−0.0235


OB2166
malate dehydrogenase
GK2734
+
312
−0.0139


OB1414
pyruvate dehydrogenase E2
GK1060
+
427
−0.0102


OB0010
inosine-5′-monophosphate
GK0009
+
489
−0.0137


OB1694
DNA topoisomerase IV subunit A
GK1750
+
816
−0.0149


OB1896
Xaa-Pro dipeptidase
GK2411
+
353
−0.0144


OB1367
hypothetical protein
GK1982
+
178
−0.0148


OB1779
hypothetical protein
GK2195
+
420
−0.0111


OB2118
electron transfer flavoprotein alpha
GK2686
++
323
−0.0080


OB3225
stage V sporulation protein N
GK3448
++
376
−0.0080


OB1349
1-pyrroline-5-carboxylate
GK0187
++
515
−0.0053


OB0140
adenylate kinase
GK0127
++
215
−0.0069


OB0656
class I heat shock protein
GK0249
++
545
−0.0054


OB1968
class I heat shock protein 70
GK2504
++
612
−0.0070


OB0093
ATP-dependent Clp protease
GK0078
++
809
−0.0077


OB1427
hypothetical protein
GK1076
++
149
−0.0067


OB2359
hypothetical protein
GK2967
++
172
−0.0057


OB0002
DNA-directed DNA polymerase III beta
GK0002
+++
378
0.0103


OB2380
ABC transporter ATP-binding protein
GK2995
+++
261
−0.0021


OB2117
thioredoxin
GK2685
+++
104
0.0068


OB2119
electron transfer flavoprotein beta
GK2687
+++
257
−0.0005


OB2975
H(+)-transporting ATP synthase beta
GK3358
+++
464
0.0026


OB1483
cell-division initiation protein
GK1135
+++
167
0.0008


OB2475
glycerol kinase
GK1360
+++
500
0.0065


OB1415
pyruvate dehydrogenase E3
GK1061
+++
468
0.0061


OB1090
2-oxoglutarate dehydrogenase E2
GK1024
+++
422
0.0259


OB1543
class I heat shock protein
GK1208
+++
386
0.0020


OB2167
isocitrate dehydrogenase (NADP+)
GK2735
+++
422
0.0020


OB2388
Glycine cleavage system H protein
GK3004
+++
126
0.0003


OB1787
nucleoside-diphosphate kinase
GK2209
+++
148
0.0111


OB1886
acetyl-CoA carboxylase biotin carboxyl
GK2400
+++
159
0.0147



carrier subunit


OB1168
ferrochelatase
GK0662
+++
312
0.0109


OB2590
DNA topoisomerase III
GK1688
+++
720
−0.0019


OB1551
transcriptional pleiotropic repressor
GK1215
+++
259
−0.0015


OB3452
two-component response regulator
GK3474
+++
233
−0.0014


OB0060
50S ribosomal protein L25
GK0045
+++
215
0.0037


OB0110
50S ribosomal protein L7/L12
GK0096
+++
120
0.0004


OB0116
translation elongation factor EF-G
GK0103
+++
692
0.0024


OB0117
elongation factor EF-Tu
GK0104
+++
395
0.0064


OB1587
elongation factor EF-Ts
GK1250
+++
294
0.0280


OB1410
formylmethionine deformylase
GK1057
+++
183
−0.0011


OB1508
hypothetical protein
GK1175
+++
254
0.0078


OB0655
class I heat shock protein
GK0248
+++
93
−0.0036


OB2078
trigger factor
GK2653
+++
428
0.0054


OB1932
manganese superoxide dismutase
GK2457
+++
203
0.0040


OB1444
hypothetical protein
GK1089
+++
121
−0.0010


OB3023
hypothetical protein
GK3416
+++
249
0.0376







Difference in scores of principal component analysis between gk and ob





−: <−0.015 to be judjed as lack of thermostability





+: >−0.015 to be judged to have thermostability





++: >−0.010 to be judged to have thermostability





+++: >−0.005 to be judged to have thermostability














TABLE 7










List of thermostable proteins from Bacillus cereus confirmed experimentally and its


comparison with computational prediction of the thermostability

















Difference in scores




Corresponding


of principal


Gene name of

gene name of
Result of
Number of amino
component analysis


BC
Product name
GK
Prediction
aids of the product
between gk and bc















BC0152
Adenylate kinase
GK0127

215
−0.0200


BC0294
10 kDa chaperonin GroES
GK0248

95
−0.0213


BC1510
DNA-binding protein HU
GK2215

113
−0.0231


BC4471
Porphobilinogen deaminase
GK2645

308
−0.0213


BC2488
Propionyl-CoA carboxylase beta chain
GK1603
+
512
−0.0116


BC4163
Phosphate butyryltransferase
GK2382
+
298
−0.0123


BC0013
Inosine-5′-monophosphate dehydrogenase
GK0009
++
486
−0.0068


BC1021
CMP-binding factor
GK0646
++
313
−0.0094


BC4523
Electron transfer flavoprotein beta-subunit
GK2687
++
256
−0.0093


BC4571
Deblocking aminopeptidase
GK2713
++
362
−0.0062


BC0102
Negative regulator of genetic competence
GK0078
+++
810
−0.0034


BC0108
Glutamyl-tRNA synthetase
GK0083
+++
495
0.0051


BC0110
Cysteinyl-tRNA synthetase
GK0085
+++
464
0.0055


BC0295
60 kDa chaperonin GROEL
GK0249
+++
543
−0.0012


BC0377
Alkyl hydroperoxide reductase C22
GK2575
+++
186
−0.0027


BC0380
L-fuculose phosphate aldolase
GK1906
+++
212
0.0211


BC0778
Thioredoxin
GK0567
+++
149
0.0215


BC1127
Malate synthase
GK1533
+++
519
0.0214


BC1168
ClpB protein
GK0799
+++
865
0.0068


BC1338
Oligoendopeptidase F
GK0963
+++
563
0.0062


BC1406
Histidinol dehydrogenase
GK3075
+++
428
0.0034


BC1511
GTP_cyclohydrol, GTP cyclohydrolase I
GK2214
+++
188
0.0003



Non-specific DNA-binding protein Dps/


BC2011
Iron-binding ferritin-like antioxidant
GK2861
+++
146
0.0084



protein/Ferroxidase


BC2778
Acetoin dehydrogenase E1 component
GK0711
+++
343
−0.0032


BC2833
Dihydrodipicolinate synthase
GK1961
+++
297
0.0414


BC3652
Histidine ammonia-lyase
GK0385
+++
505
0.0112


BC3824
Protein Translation Elongation Factor Ts
GK1250
+++
294
0.0094


BC4162
Leucine dehydrogenase
GK2381
+++
365
0.0043


BC4198
Xaa-Pro dipeptidase
GK2411
+++
352
−0.0028


BC4312
Chaperone protein dnaK
GK2504
+++
610
0.0057


BC4600
6-phosphofructokinase
GK2740
+++
318
−0.0017


BC4661
Acetoin utilization acuB protein
GK2808
+++
213
0.0080


BC4702
Xaa-His dipeptidase
GK2831
+++
467
0.0005


BC4902
Transcriptional regulator, AsnC family
GK2929
+++
164
0.0042


BC5190
Probable Sigma (54) modulation protein
GK3109
+++
179
0.0090


BC5280
(3R)-hydroxymyristoyl-[acyl carrier
GK3329
+++
143
0.0309



protein] dehydratase


BC5343
3-hydroxybutyryl-CoA dehydrogenase
GK3395
+++
272
0.0041


BC5474
S30P Probable Sigma (54) modulation
GK3480
+++
76
0.0117



protein/SSU ribosomal protein







Difference in scores of principal component analysis between gk and bc





−: <−0.015 to be judged as lack of thermostability





+: >−0.015 to be judged to have thermostability





++: >−0.010 to be judged to have thermostability





+++: >− to be judged to have thermostabitity







Tables 4 to 7 show the details of proteins confirmed to have thermostability by the heat treatment study, which were derived from B. subtilis (BS) (Table 4), B. halodurans (BH) (Table 5), O. iheyensis (OI) (Table 6), and B. cereus (BC) (Table 7), respectively. The columns of the respective tables indicate, from the left, “gene name of BS, BH, OI or BC”, “product name thereof”, “corresponding gene name of GK”, “result of prediction”, “number of amino acids of the product”, and “difference in scores of principal component analysis between GK and BS, BH, OI or BC”, respectively. In the column of “result of prediction”, “−” indicates the case where the difference in PC2 values between each microorganism and GK is lower than −0.015, thereby being judged lack of thermostability, and “+”, “++”, “+++” indicate the cases where the difference is greater than −0.015, −0.01 and −0.005, respectively, thereby being judged presence of thermostability.


As shown in Tables 4 to 7, at least 38 thermostable proteins for BC and BH, 117 thermostable proteins for BS and 52 thermostable proteins for OI were identified. Then, how the presence of or lack of thermostability of the proteins, which were confirmed to have thermostability had been predicted by comparison of the principal component scores between GK and other Bacillus-related species was investigated. As described above, when the difference in the principal component scores between the respective Bacillus-related species and GK≧−0.015 is defined to have thermostability, it is found that 34 out of 38 proteins (89.5%) for BC shown in Table 7, 36 out of 38 proteins (94.7%) for BH shown in Table 5, 103 out of 117 proteins (88.0%) for BS shown in Table 4, and 46 out of 52 proteins (88.5%) for OI shown in Table 6 were predicted to have thermostability by the method of the invention.


These results are summarized and shown in the following Table 8. The respective signals in Table 8 are the same as in Table 2. Accordingly, the method of the invention capable of judging the thermostability of a protein produced by a mesophilic bacterium by calculating the correlation with a corresponding protein of a thermophilic bacterium indicates the thermostability of the protein.

TABLE 8BCBHBSBSOIprediction(number)BC (%)(number)BH (%)(number)(%)(number)OI (%)410.525.31412.0611.5+25.3410.52017.1713.5++410.5718.41412.0917.3+++2873.72565.86959.03057.7++, +++3284.23284.28370.93975.0+, ++, +++3489.53694.710388.04688.5total383811752


The method of the invention was explained based on the Bacillus-related species. However, it is easily understood by those skilled in the art that the method of the invention is not limited to the Bacillus-related species, and can be applied to any species as long as a thermostable protein corresponding to a test protein exists.


A “thermostable organism” in the invention may be an organism that can maintain its life at a temperature where human can maintain his/her life or higher, however, the term is referred to as an organism that can maintain its life at specifically about 50° C. or higher, preferably 60° C. or higher, more preferably 65° C. or higher. Examples include thermophilic bacteria, spring organisms and the like. As the “thermostable organism” in the method of the invention, a thermostable organism which has a relationship with an organism producing a test protein is preferred. As the “relationship” referred to here, similarity in a biological classification, genetic similarity in embryology, functional similarity retained by the test protein and the like can be exemplified.


A “protein retained by a thermostable organism” in the invention is a protein produced by a thermostable organism, and may be any protein as long as it is produced by a thermostable organism whether or not it is essential to life.


In addition, a “protein which is retained by a thermostable organism and corresponds to a test protein” in the invention may be a protein with the same type of function as that of a test protein, preferably with the function equal to that of a test protein. It is not necessary to have a biological or embryological relationship, however, a protein with a biological or embryological relationship may be preferably exemplified. For example, as described above, a correlation based on a biological orthologous gene, a correlation of proteins with the same type of function among organisms of the same genus or the same species, etc. are exemplified.


The “protein which is retained by a thermostable organism and corresponds to a test protein” in the method of the invention is not always one protein, and may be 2 or more proteins. In the case where 2 or more proteins can be selected as such a protein, it is possible to compare these one another, and to perform judgment comprehensively.


As the method of calculating a “thermostability index of a test protein based on the amino acid composition” in the method of the invention, a method based on a principal component analysis comprising the steps of extracting a protein based on a gene encoding a protein, which is identified in the genome of an organism as described above as an example, excluding a protein whose amino acid sequence length is less than 50 amino acids from these proteins, further excluding a protein which has been predicted to contain 2 or more transmembrane domains by the PSORT program, calculating an average amino acid composition on a species basis by using the amino acid sequences of the remaining proteins, and with regard to the calculated average amino acid composition, using the princomp function in the R statistical analysis package by using a matrix, as input, in which each row and column corresponds to the species and an amino acid, respectively (Kreil D. P. and Ouzounis, C. A. (2001), Identification of thermophilic species by the amino acid compositions deduced from their genome. Nucleic Acids Res. 29, 1608-1615) is effective. However, the method is not limited thereto, and if there are predetermined number or more of proteins whose thermostability has been verified experimentally, it is possible to improve the method by incorporating a technique such as a discrimination analysis or a regression analysis. In addition, it is preferred to use an entire protein (whole length) in the invention, however, it is possible to use each domain or a partial length of a protein as a target.


As the “comparison of analytical values” in the method of the invention, a method of obtaining a difference between the analytical values as described above is convenient and preferred, however, it is not limited thereto. In the case where a large amount of data is accumulated, it is possible to perform comparison based on a difference with the average value of all elements or a value processed statistically such as deviation.


In addition, a judgment criterion in the comparison can be set within a range where it can be confirmed that a test protein has thermostability practically. In the foregoing example, it can be judged that a protein has thermostability when a difference in principal component scores calculated by the value of an eigenvector (weighting factor of each amino acid) and the number of amino acids of each protein is in a range of about 0.005 to 0.015 or lower. Such judgment is not only represented by the presence of or lack of thermostability, but can be represented by a ratio (%) of the possibility of having thermostability.


As the data for calculating a specific analytical value by a principal component analysis based on the amino acid composition of a test protein in the method of the invention, data of the amino acid sequence or the nucleotide sequence of the protein and the like are exemplified, however, it is not limited thereto and may only be its amino acid composition. As such data, in order to increase judgment accuracy, data with a large amount of information is preferred, however, the nucleotide sequence encoding the protein as described above as an example can be cited as a convenient and preferred example. Other than this, three-dimensional data of a protein can be further added, however, what data is required depends on not only improvement of judgment accuracy but also an approach for processing the data.


Specifically, the method of the invention comprises the following steps (1) to (6):

    • (1) a step of obtaining the amino acid sequence of a protein and/or the nucleotide sequence encoding the protein,
    • (2) a step of calculating the “specific analytical value” of the protein based on the data of the amino acid sequence and/or the nucleotide sequence,
    • (3) a step of selecting a “protein which is retained by a thermostable organism and corresponds to a test protein” by using the protein as the test protein,
    • (4) a step of obtaining data of the analytical value of the selected “corresponding protein”,
    • (5) a step of comparing both analytical values, and
    • (6) a step of performing judgment based on the results of comparison.


With regard to these steps, except for the determination of the sequence in the step (1) and the selection in the step (3), their processing methods can be specified in advance, and processing in a computer is possible. In addition, with regard to the step (3), if classification has been performed in advance based on an enzyme classification, a “corresponding protein” which is a subject to be selected can be selected from accumulated data. Accordingly, all the steps except for the step (1) can be processed in a computer.


In other words, in the invention, the method of the invention described above is programmed so as to be processed in a computer, and the invention provides a processing method in a computer comprising (a) a method of calculating a specific analytical value by processing in a computer by inputting data of the amino acid sequence or the nucleotide sequence of the protein into the program, (b) a method of extracting a “corresponding protein” to the protein from accumulated data based on the classification signal, function data, origin data or the like, (c) a method of referring to the specific analytical value of the “corresponding protein” extracted in the step (b) as a value of calculated or accumulated data, (d) a method of comparing the specific analytical value of the protein and the specific analytical value of the “corresponding protein”, and (e) a method of displaying (outputting) the result of comparison.


In the processing in a computer, the analytical value of a protein which is retained by a thermostable organism and corresponds to a test protein can be calculated in each case, however, it is also possible that a value calculated by a principal component analysis based on the amino acid composition of the protein is classified according to the type of each protein and listed to create accumulated data. Such accumulated data can be stored in a computer readable recording medium so as to utilize it as the information for processing in a computer. Examples of such a recording medium include a hard disk, DVD disc, CD-ROM, MO, floppy disc and the like.


As the program of the invention for judging whether or not a test protein has thermostability by allowing a computer to execute each of the following steps, for example a program for judging whether or not a test protein has thermostability by comparing a specific analytical value based on the amino acid composition of a test protein and a specific analytical value of a known corresponding protein by the steps of:

    • (1) inputting the amino acid sequence of the test protein,
    • (2) searching a known protein related to a corresponding protein produced by another species different from the one producing the test protein (corresponding protein),
    • (3) calculating a specific analytical value by a principal component analysis based on the amino acid composition of the test protein,
    • (4) calculating the specific analytical value of the corresponding protein searched in the step (2) and the specific analytical value of the test protein calculated in the step (3), and calculating the difference between both values,
    • (5) judging whether or not the test protein is similar to the corresponding protein searched in the step (2) based on the difference calculated in the step (4), and
    • (6) displaying the corresponding protein searched in the step (2) and the result of judgment in the step (5)


      is exemplified.


Hereunder, the program of the invention will be explained. In the following, explanation will be made by using a protein which is in an orthologous relationship as an example of the corresponding protein, and a second principal component score of the principal component analysis as an example of the specific analytical value based on the amino acid composition. In addition, the program of the invention can be executed as a stand-alone program, however, in the following, explanation will be made by using a server-type program as an example. The following explanation is only an example of the invention, and the invention is not limited to these examples.



FIG. 8 shows an execution flowchart of the client. When it starts up, the startup screen is displayed, and data necessary for an orthologue search is read. After startup setting is completed, the screen for input from a terminal is displayed. The input of a test protein may be performed by any method such as type in, FD, CD and online, and the amino acid sequence and/or the nucleotide sequence of a test protein and its origin are input. In FIG. 8, they are indicated as a “variable plot”.


After completing the input, an orthologue search is executed, however, it is optionally designed that an organism to be searched can be selected. The selection of a species is not essential, and all the accumulated species can be also used as a target. An orthologue search is executed for a designated species.


As a method of an orthologue search, a variety of parameters such as the amino acid sequence, amino acid composition, function, origin and expressed organ of a test protein can be adopted, however, in this example, an orthologue search is executed by a homology search based on the amino acid sequence. A protein, which has a high homology to a test protein, for example, with a homology of 70% or higher, 80% or higher, or 85% or higher and is derived from a species different from that of the test protein, is selected as an orthologue candidate in this example.


In the case where a protein to become a corresponding orthologue could not be retrieved from the orthologue search result, comparison cannot be performed (in FIG. 8, “Is an orthologue list present?”→“no”), therefore the processing is finished.


In the case where one or more orthologues were retrieved (in FIG. 8, “Is an orthologue list present?”→“yes”), an orthologue list is created and a second principal component score based on the amino acid composition for each orthologue is calculated. Then, The second principal component score of the test protein and the second principal component score of the corresponding protein are compared to obtain the difference, and judgment is performed.


With regard to the judgment at this time, in this example, three stages, ±0.005, ±0.010, ±0.015 of the difference in both scores are set as default, however, a user can set it optionally. This result is displayed in an excel format or a screen display format.


This result is basically displayed in a table format, however, it can be displayed in a graph designated by a user based on this table format. In addition, depending on the degree of difference, it may be colored. In this case, as the color, red, blue, green or the like may be used to indicate default values.



FIG. 9 shows a flowchart from the server until data input. A startup request is issued by a client, a program is started, and data is read. After completing data format check, a character string other than that of an amino acid is deleted, and recognition of the amino acid is performed. Based on the input amino acid sequence, the number of amino acids is counted. In the case where the number of amino acids is less than 50, the processing is finished (In FIG. 9, “Minimum length check”). Subsequently, whether or not the input protein has a transmembrane domain is detected by the “SOSUI” program. This program is a program for deducing a transmembrane domain from the sequence of a hydrophobic amino acid. In the case where the input protein was judged to have 2 or more transmembrane domains by the “SOSUI” program, the protein is considered to be a membrane protein and excluded from the subjects of processing of this program, and the processing is finished.


In the case where the number of the amino acids of the input protein is 50 or more and the site deduced to be a transmembrane domain is one or less, an analysis of the amino acid composition is carried out. With regard to the analysis of the amino acid composition, for each of the 20 types of amino acids in the open reading frame (ORF), the ratio of content of each amino acid is calculated at a percentage. Subsequently, a principal component analysis is carried out. In this principal component analysis, a commercially available program for statistical processing can be used. A second principal component score is calculated by a principal component analysis, and data input processing is completed.


With regard to a corresponding protein search, a homology search is executed from the N-terminal side and the C-terminal side of a protein by using, for example, BLASTP, and a protein with the highest homology is defined as a corresponding protein. The case where only a protein with a homology of 70% or lower as default is searched is defined as no corresponding protein, however, the lower limit of homology can be set by a user.


The program of the invention refers to a database of known proteins for a corresponding protein search. In order to this, it is necessary to accumulate data of known proteins, therefore, the program of the invention can also include a step of inputting data of a known protein for a corresponding protein search. As a data source of such data, a paper published in an academic journal, a database available on the Internet and the like are exemplified. In the case of a database available on the Internet, it is possible to program a computer to automatically access the Internet on a regular or irregular basis and to automatically download new information. Data obtained in this way can be stored in a reference file of the program of the invention as accumulated data through the same flow as shown in FIG. 9.


In addition, the program of the invention refers to a database of the second principal component scores of a principal component analysis based on the amino acid composition of a known protein. The second principal component score can be calculated based on the amino acid sequence in the database of known proteins for a corresponding protein search. Therefore, when a known protein is input for the foregoing corresponding protein search, the score can be calculated and input as accumulated data.


The program of the invention can further include such an input step.


The main functions of the program of the invention are summarized and shown below.


The amino acid sequences of a microorganism with thermostability and of several species of closely related microorganisms without thermostability are used as input, and the results of a principal component analysis based on the amino acid compositions are displayed as a scatter chart. From the scatter chart of the principal component scores on a microorganism basis, a microorganism with thermostability can be deduced, further, an exceptional microorganism candidate whose deduction results from the actual growth temperature and the principal component analysis disagree with each other can be obtained.


By the function of comparing the second principal components of proteins in an orthologous relationship between a thermophilic bacterium and a mesophilic bacterium, a thermostable protein in a mesophilic bacterium can be deduced. In addition, in the case of an exceptional microorganism whose deduction results from the actual growth temperature and the principal component analysis disagree with each other, deduction of a gene closely related to thermostability can be performed.


Further, the program of the invention comprises two steps: one is a calculation step for creating a data set necessary for prediction of thermostability, and the other is a step of predicting thermostability based on the amino acid composition of a protein, for which the presence of or lack of thermostability is desired to be known, and the contents and the order of processing are as follows.


(1) Data Set Creation Step


(a) Minimum sequence exclusion: Exclude an amino acid sequence shorter than a predetermined length.


(b) Hydrophobic domain exclusion: Exclude a sequence containing 2 or more transmembrane domain based on the data hit by SOSUI (transmembrane domain prediction program).


(c) Determination of an orthologue among the respective species:


Execute BLASTP against all the entries, and acquire the one with the best score from the results one by one.


Create FASTA file in which only the result of orthologue was left (W1).


(d) Calculation of Amino Acid Composition:


Calculate an amino acid composition on an orthologue basis, and calculate the average on a species basis.


Execute calculation based on W1 File. Store the amino acid compositions on an orthologue basis as W2 file.


(e) Principal component analysis: Calculate a principal component score based on the amino acid composition.


Based on the principal component score on a species basis, output the display data for a scatter chart of the principal component scores into W3 file.


By using the eigenvector of the second principal component and W2 file, calculate the score for each orthologue and store it in W4 file.


(2) Thermostability Prediction Step


(a) Display of the whole distribution chart:


Read I2, I3 and W3 files, and create and display a scatter chart on a species basis (each parameter can be selected).


From the whole distribution chart, a reference organism (an organism having a corresponding protein) and a comparable species (the plural organisms is also applicable) can be selected.


(b) Compare the scores of proteins in an orthologous relationship among all the proteins of an organism having a corresponding protein and an organism having a test protein.


(c) With regard to the selected species, read W1 and W4 files and obtain the information.


(d) Display a list of the differences in the scores of the proteins in an orthologous relationship among all the proteins retained in an organism having a corresponding protein and the respective comparative species (depending on the difference degree, the differences are distinguished by using three different colors).


(e) In addition, display the differences in the scores of orthologues showing one-to-one correspondence of an organism having a corresponding protein and a comparative organism as a scatter chart.


The main functions of the program of the invention are summarized and shown in the following Table 9.

TABLE 9Name of functionContents1Input data creation supportFunction of automatically downloading a default formatfunctionand further supporting creation of an input file of asystem.2Parameter control functionFunction of setting and storing a processing method ofexecuting project data creation processing and orthologuesearch processing3Input data check functionFunction of executing, with regard to the input data, (1)format check, (2) deletion of unnecessary character string,(3) length check, and (4) exclusion of hydrophobic aminoacid sequence.4Principal component analysisFunction of calculating the amino acid composition offunctioneach microorganism, and executing a principal componentanalysis based on the results.5Display function of scatter chartFunction of displaying the principal component analysisof principal component analysisresults as a scatter chart, and further outputting the imageresultsof the scatter chart as an image file in an editable layer.6Orthologue search functionFunction of detecting an orthologue amongmicroorganisms selected by a user by executing simplexor duplex BLAST.7Orthologue list creation functionFunction of displaying an orthologue list and the secondprincipal component score for each orthologue and thescore after comparison. Direct printing from the screenor output in an Excel format can be performed.8Display function of orthologueFunction of displaying the second principal componentscatter chartscores for each orthologue between 2 organisms as ascatter chart, and further outputting the image of thescatter chart as an image file in an editable layer.9Input function of sequence ofFunction of executing processing corresponding to inputcomparisondata check function and orthologue search function withregard to the plural amino acid sequences input in MultiFastA format from the screen, and further calculating thesecond principal component scores and displaying the listand the scatter chart.


The program of the invention can be stored on a computer readable recording medium in order to allowing a computer to execute the program. Examples of such a recording medium include a hard disk, DVD disc, CD-ROM, MO, floppy disc and the like.


Therefore, the invention also provides a computer readable recording medium having stored thereon the program of the invention.


In the recording medium of the invention, a database of known proteins and a database of specific analytical values based on the amino acid compositions of known proteins for a corresponding protein search, which the program of the invention refers to, can be recorded.


The method of the invention enables prediction of the thermostability of a protein by calculating a specific analytical value of the protein without conducting an experiment, or more conveniently, on a personal computer, therefore, it is very rapid and inexpensive. In addition, the invention enables the judgment not on a basis of an organism, but on a basis of a protein produced by the organism. Therefore, the search scope of a thermostable enzyme whose source was conventionally limited to a thermophilic bacterium can be extended to the scope of a protein produced by a mesophilic bacterium, whereby the range of screening for thermostable proteins can be expanded. Further, with regard to the screening of a thermostable enzyme from a mesophilic bacterium which had taken enormous time and effort before, since candidates of thermostable enzymes can be narrowed down in advance, whereby it becomes possible to easily perform search or screening of a thermostable enzyme, which can be applied to various processes.


Further, by using the computer program developed by the invention, a thermostable protein derived from a mesophilic bacterium closely related to a thermophilic bacterium is conveniently predicted, whereby it is possible to shorten the time required for a search of a wider variety of thermostable enzymes than ever to a large extent. In addition, the program of the invention enables prediction of the thermostability of a protein for which the presence of or lack of thermostability is desired to be known on a personal computer working with Windows™, therefore, it can be easily used by, in particular, even a person who has no knowledge of computer language.


Hereunder, the invention will be explained more specifically with reference to the Examples, however, the invention is by no means limited to these Examples.


EXAMPLES
Example 1

Calculation Method of Data of 120 Species of Bacteria


From the database at NCBI, the genome data of 119 species of microorganisms was obtained, and the sequences of proteins identified in the 120 types of genomes including the obtained 119 types of genomes and the genome of G. kaustophilus HTA426, which had been determined in the invention were used for an analysis. From these sequences of proteins, a protein with a sequence length of less than 50 amino acids was excluded, further a protein which had been predicted to contain 2 or more transmembrane domains by the PSORT program (K. Nakai, P. Horton, Trends Biochem. Sci., 24, 34-6, 1999) was also excluded. By using the sequences of the remaining proteins, an average amino acid composition was calculated on a species basis, a matrix in which each row and column corresponds to a species and an amino acid, respectively was input, and a principal component analysis was performed in accordance with the method of Kreil et al. (D. Kreil, C. Ouzounis, Nucleic Acids Res, 29, 1608-15, 2001). In the analysis, the princomp function in the R statistical analysis package was used.


Example 2

Calculation Method of Data of Specific Analytical Values of 965 Proteins


Orthologous grouping of 5 species of microorganisms, GK, BC, BH, BS and OI was performed using the clustering program on MBGD (I. Uchiyama, Nucleic Acids Res, 31, 58-62, 2003) server by Uchiyama. Only an orthologous group present in all the 5 species and showing one-to-one correspondence was used for the analysis. Further, a group containing 4 or more proteins which had been predicted to contain 2 or more transmembrane domains by PSORT was excluded. By using the eigenvector of the second principal component obtained in the principal component analysis described in Example 1, the thermostability index of each protein was calculated as an inner-product of the amino acid composition vector with the eigenvector.


Example 3

Analysis of all the Proteins


A liquid culture was performed aerobically for 18 hours by using LB medium (pH 7) for GK, BS and BC, and Horikoshi II medium (pH 9.5) (Takami, H, Kobayashi, T., Aono, R., and Horikoshi, K. Appl. Microbiol. Biotechnol. 38, 101-108, 1992) for BH and OI. The culture was performed at 55° C. for GK and at 37° C. for the other microorganisms. The cultured cells were harvested by centrifugation, washed with 50 mM phosphate buffer, and resuspended in the same buffer, whereby a cell suspension was obtained. Then, the cell suspension was subjected to a French press, and the obtained homogenized cell suspension was centrifuged to remove the cell debris. The obtained supernatant was used as a protein solution for the analysis of all the proteins. In addition, this protein solution was treated with heat at 60° C. or 70° C. for 10 minutes, then rapidly cooled down to obtain a heat-treated protein solution. The analysis of all the proteins was carried out by native gel electrophoresis. The gel concentration was 12.5%. After the electrophoresis, the gel was stained with Coomassie Brilliant Blue.


Example 4

Identification of Thermostable Protein


By using the protein solutions of the respective organisms prepared by the method described in Example 3, the proteins were separated by native gel electrophoresis, stained with Coomassie Brilliant Blue in the same manner as in Example 3. From the lanes 3 of 4 species except for GK in FIG. 6, which were obtained by subjecting the protein solutions treated with heat at 70° C. for 10 minutes to electrophoresis, the bands of proteins that were not lost after the heat treatment were cut out from the gel with a length of 3 mm each. Then, in accordance with the usual methods, the proteins in the gel were treated with trypsin, and the peptides were fractionated by an LC/MS/MS system, whereby the mass was calculated. The mass analysis was carried out by using Bioworks 3.1, Xcalibour system manufactured by Thermo Electron Co., and comparing the results and the database of the proteins of each Bacillus-related species. In this way, identification of the proteins contained in each band was carried out.


The results are shown in Tables 4 to 7.


Example 5

Analysis of Esterase


By using the protein solutions of the respective organisms prepared by the method described in Example 3, the proteins were separated by native gel electrophoresis in the same manner. Then, detection of only the band having an esterase activity was carried out by the method shown below.


Two milliliter of 1% α-naphtyl acetate dissolved in 50% acetone and 100 mg of fast blue BB salt were added to 100 ml of 0.05 M Tris-HCl buffer (pH 7.4), mixed well, and the solution was transferred to a plastic container. Then, the gel after the electrophoresis was immersed in the solution and incubated at 37° C. for 10 minutes in the dark. When the band having an esterase activity appeared, the solution was removed, and the gel was washed with distilled water.


By using the obtained esterase from each organism, a protein solution without heat treatment, protein solutions with heat treatment at 60° C. and 70° C. for 10 minutes, which had been rapidly cooled down after the heat treatment, were prepared, and native gel electrophoresis was carried out. The gel concentration was 12.5%.


Example 6

Analysis of Flagellin


By using a primer set designed from the nucleotide sequences of hag genes of the 5 strains, the hag genes were amplified by PCR. Then, these PCR products were ligated to a plasmid vector for TA cloning with His-tag at the N-terminal end (pCRT7 TOPOTA), and transformation of E. coli (E. coli BL21 DE3) was carried out. The transformed E. coli was cultured until OD 600 reached 0.6. Then, 0.5 mM IPTG was added and the protein was expressed at 30° C. for 3 to 5 hours. The cells were homogenized with a French press in the same manner as above, and the obtained homogenized cell suspension was applied to a Talon metal affinity column for conveniently purifying only a protein with His-tag, and the protein was allowed to adhere to the column. Then, the target protein was purified with 150 mM imidazole, 50 mM sodium phosphate and 300 mM NaCl. The purified protein was subjected to SDS-PAGE electrophoresis and the degree of purification was confirmed.


By using the purified protein, heat treatment was carried out in accordance with the method described in Example 4. Then, the proteins were separated by native gel electrophoresis, and stained with Coomassie Brilliant Blue.


Example 7

Analysis of GroES


By using a primer set designed from the nucleotide sequences of groES genes of the 5 strains, the groES genes were amplified by PCR. Then, the proteins were produced and purified in the same manner as in Example 6. In addition, by using the purified protein, heat treatment and electrophoresis were carried out in the same manner, whereby analysis of GroES protein was carried out.


A thermostable protein such as a thermostable enzyme is utilized in various industrial fields such as sugar industry, protein industry and fertilizer industry, and its importance is extremely high. In addition, as a DNA polymerase or the like, it is considered to be indispensable to use a thermostable enzyme in genetic engineering techniques.


The method of the invention provides a novel method of searching a thermostable protein such as a thermostable enzyme by a convenient approach, and is an extremely useful method in industry. In addition, the method of the invention indicates that the search scope of thermostable proteins can be further expanded from the conventional proteins derived from thermophilic bacteria, and makes an extremely significant contribution in industry.

Claims
  • 1. A method of judging the thermostability of a protein, which judges whether or not a test protein has thermostability, comprising the steps of calculating an analytical value specific to the test protein by a principal component analysis based on the amino acid composition of the protein, and comparing the analytical value with an analytical value of a protein which is retained by a thermostable organism and corresponds to the test protein.
  • 2. The method according to claim 1, wherein the specific analytical value by the principal component analysis based on the amino acid composition of the test protein is calculated based on data of the amino acid sequence or the nucleotide sequence of the protein.
  • 3. The method according to claim 2, wherein a method of calculating the specific analytical value by the principal component analysis based on the amino acid composition of the protein is programmed so as to be processed in a computer, and the data of the amino acid sequence or the nucleotide sequence of the protein is input into the program, whereby the specific analytical value is calculated by processing in a computer.
  • 4. The method according to claim 1, wherein a method of calculating the analytical value of the protein which is retained by a thermostable organism and corresponds to the test protein, is in accordance with the method according to claim 2 or 3.
  • 5. The method according to claim 1, wherein the analytical value of the protein which is retained by a thermostable organism and corresponds to the test protein, is calculated by the principal component analysis based on the amino acid composition of the protein, and listed according to the category of each protein.
  • 6. The method according to claim 1, wherein the list of the analytical values according to claim 5 is stored in a computer processable recording medium in such a manner that the list can be used as information for processing in a computer.
  • 7. The method according to claim 1, wherein the comparison of the analytical value specific to the test protein with the analytical value of the protein which is retained by a thermostable organism and corresponds to the test protein, is carried out by processing in a computer.
  • 8. The method according to claim 1, wherein the principal component analysis based on the amino acid composition of the protein comprises the steps of extracting a gene encoding a protein, which has been identified in the genome of an organism, excluding a protein whose amino acid sequence length is 50 amino acids or less based on the amino acid sequence of the protein encoded by the gene, further excluding a protein which has been predicted to contain 2 or more transmembrane domains by the PSORT program, calculating an average amino acid composition on a species basis by using the amino acid sequences of the remaining proteins, and using the princomp function in the R statistical analysis package by using, as input, a matrix in which each row and column corresponds to the species and an amino acid, respectively.
  • 9. The method according to claim 1, wherein the thermostable organism is a thermophilic bacterium.
  • 10. The method according to claim 1, wherein the protein, which is retained by a thermostable organism and corresponds to the test protein, is in a biologically orthologous relationship with the test protein.
  • 11. The method according to claim 1, wherein the protein is an enzyme.
  • 12. The method according to claim 1, wherein the protein is produced by a microorganism belonging to the genus Bacillus or Bacillus-related species.
  • 13. A program for allowing a computer to execute processing for judging the thermostability of a protein, which allows a computer to execute judgment whether or not a test protein has thermostability, by calculating an analytical value specific to the test protein by a principal component analysis based on the amino acid composition of the protein, and comparing the analytical value with an analytical value of a protein which is retained by a thermostable organism and corresponds to the test protein.
  • 14. The program according to claim 13, which allows a computer to judge whether or not a test protein has thermostability by executing the steps of: (1) inputting the amino acid sequence of the test protein, (2) searching a known protein related to a corresponding protein produced by another species different from the one producing the test protein (hereinafter referred to as corresponding protein), (3) calculating a specific analytical value by a principal component analysis based on the amino acid composition of the test protein, (4) calculating the specific analytical value of the corresponding protein searched in the step (2) and the specific analytical value of the test protein calculated in the step (3), and calculating the difference between both values, (5) judging whether or not the test protein is similar to the corresponding protein searched in the step (2) based on the difference calculated in the step (4), and (6) displaying the corresponding protein searched in the step (2) and the result of judgment in the step (5), whereby the specific analytical value based on the amino acid composition of the test protein and the specific analytical value of the known corresponding protein are compared to judge whether or not the test protein has thermostability.
  • 15. The program according to claim 14, wherein the relationship of the corresponding protein produced by another species different from the one producing the test protein (corresponding protein) is an orthologous relationship.
  • 16. The program according to claim 13, wherein the specific analytical value based on the amino acid composition of the protein is an analytical value of a second principal component in the principal component analysis.
  • 17. The program according to claim 14, further comprising a step of checking whether or not the protein is a subject of processing.
  • 18. The program according to claim 14, wherein the protein which is a subject of processing comprises 50 or more amino acids and contains one or less transmembrane domain.
  • 19. The program according to claim 14, further comprising a step of inputting data of a known protein for a corresponding protein search.
  • 20. The program according to claim 14, further comprising a step of inputting a specific analytical value based on the amino acid of a known protein.
  • 21. A computer readable recording medium having recorded thereon a program for allowing a computer to execute the program according to any one of claims 13 to 20.
  • 22. The recording medium according to claim 21, further having recorded thereon data of a known protein necessary for the corresponding protein search.
  • 23. The recording medium according to claim 21, further having recorded thereon data of a specific analytical value based on the amino acid composition of a known protein.
Priority Claims (2)
Number Date Country Kind
2004-046880 Feb 2004 JP national
2004-064360 Mar 2004 JP national