JP4961504B1 - New variety - Google Patents

Abstract

[Problem] To provide a new rice cultivar that can be cultivated in northern regions.
A rice cultivar Koshihikari Kazusa No. 6 having a receipt number of FERM AP-22175, an individual of the cultivar described above, and an individual progeny of the cultivar described above A progeny individual obtained by mating two individuals selected from the group consisting of
[Selection figure] None

Description

  The present invention relates to a new cultivar produced by a non-genetic recombination method, a method for distinguishing the new cultivar, and a method for premature rice plants.

  A group that belongs to the same species but has a different genetic composition and is different from other groups in a certain trait is called a breed. That is, even if it is the same kind of plant, the difficulty of cultivation, resistance to pest damage, yield, quality, and the like differ depending on the variety. For this reason, in crops, especially major crops such as rice and wheat, varieties have been improved to obtain better varieties since ancient times. In recent years, not only seed companies, but also countries and prefectures. It has also been actively conducted in the public institutions.

  With recent advances in nucleic acid analysis technology and the like, genes of various plants such as Arabidopsis thaliana, rice and wheat have been analyzed, and the gene information obtained has been disclosed. Many of these varieties have been improved by introducing a gene of a foreign species by a genetic recombination method using the disclosed gene information. For example, an Hd1 gene encoding a plant-derived protein having a function of increasing plant photosensitivity, a method for producing a transformed plant into which the Hd1 gene has been introduced, and the like have been disclosed (for example, see Patent Document 1). However, although breeding by genetic recombination has the advantage that a trait of a distantly related species that cannot normally be crossed can be introduced, there is a problem that its safety verification is not always sufficient.

  For this reason, in edible plants such as rice, many new varieties are produced by non-genetic recombination methods. For example, in Patent Document 2, when a foreign useful chromosome fragment is replaced by a non-genetic recombination method, the substitution region of the introduced foreign variety-derived chromosome fragment is controlled, and the preferred character of the original variety is changed. Without disclosing a method for producing a new variety having a target trait. Similarly, Patent Document 2 describes a new rice variety Koshihikari eichi 3 in which only the region containing the Hd1 gene of Habataki was introduced into Koshihikari by the method for producing this new variety.

  In particular, in rice, Koshihikari, which has a wider cultivatable area, is desired. Koshihikari has a better taste than other varieties and is preferred by consumers. For this reason, rice farmers prefer to cultivate Koshihikari even in areas that are not necessarily suitable for cultivating Koshihikari. However, when Koshihikari is cultivated in the southern region, the heading time is too early and a sufficient yield cannot be expected. In addition, the high taste continues during the heading season, which reduces the taste. On the other hand, when Koshihikari is cultivated in the northern region, it becomes late growth, and even if it can be headed, ripening becomes poor due to low temperature, and rice cannot be harvested.

Japanese Patent No. 3660967 Japanese Patent No. 4409610

  As a result of the study by the present inventor, it has been found that Koshihikari is only suitable for cultivation within the range of 35.5 to 38.5 degrees north latitude of Japan. If there is Koshihikari that can be cultivated in an area north of 38.5 degrees north latitude, for example, Koshihikari can be harvested even in areas that could not be cultivated conventionally, such as Hokkaido.

  It is an object of the present invention to provide a new rice cultivar that can be cultivated in the northern region of the past and a method for quickly growing rice individuals.

  As a result of diligent research to solve the above problems, the present inventor has found that a chromosome fragment of a specific region existing on the third chromosome of rice variety Habataki and a chromosome of a specific region existing on the sixth chromosome of rice variety Habataki. By substituting the fragment with the rice cultivar Koshihikari, it was found that it was possible to grow early enough to be cultivated in the northern region more than before, and the present invention was completed.

That is, the present invention
(1) Rice cultivar Koshihikari Kazusa No. 6 having an accession number of FERM P- 22175 (Oryza sativa L. multivar Koshihikari-kazusa6 gou),
(2) A progeny individual obtained by mating two individuals selected from the group consisting of an individual of the variety described in (1) and a progeny individual of the individual of the variety described in (1),
Is provided.

  Rice cultivar Koshihikari Kazusa No. 6, which is a new variety of the present invention, is much faster than Koshihikari, and can be cultivated and harvested in regions north of 38.5 degrees north latitude. In addition, rice cultivar Koshihikari Kazusa No. 6 is a new variety that is almost equivalent to Koshihikari in characteristics other than the harvest period such as quality and yield.

It is the figure which showed the target area | region T on the chromosome G of the original cultivar, the substituted foreign cultivar-derived chromosome fragment L, and the DNA markers M1 to M5. It is the figure which represented typically the genome of Koshihikari and Koshihikari eichigo No.5. It is the figure which showed the result of having investigated the heading time of Koshihikari and Koshihikari eichi No. 5 in Chiba Prefecture. It is the figure which showed the result which investigated the heading time of Koshihikari and Koshihikari eichi No. 5 in Hokkaido. It is the figure which represented typically the genome of Koshihikari eichi 3go. In Chiba Prefecture, it is the figure which showed the result of having investigated the heading time of Koshihikari and Koshihikari eichi 3go. In Hokkaido, it is the figure which showed the result which investigated the heading time of Koshihikari and Koshihikari eichi 3go. It is the figure which represented typically the genome of Koshihikari Kazusa No. 6. In Chiba Prefecture, it is the figure which showed the result which investigated the heading time of Koshihikari kazusa 6 with the result of Koshihikari, Koshihikari eichi 5 and koshihikari eichi 3. It is the figure which showed the result which investigated the heading time of Koshihikari kazusa No. 6 in Hokkaido with the result of Koshihikari, Koshihikari eichi No. 5 and Koshihikari eichi No. 3.

  In the present invention, the chromosome fragment replacement line means a line in which only a part of the chromosome of the original variety is replaced with a chromosome fragment derived from a foreign variety. Here, the foreign cultivar is not particularly limited as long as it is a cultivar other than the original cultivar, and may be a plant cultivar of the same species as the original cultivar, or a plant cultivar of a species different from the original cultivar. It may be a variety other than plants such as animals. In the present invention, the cultivar means a group that can be clearly distinguished from other varieties in the same species in a certain trait because the plants are of the same species and have different genetic constitutions.

  In the present invention, the DNA marker is not particularly limited as long as it can detect the difference in the DNA sequence on the chromosome that can distinguish the chromosome derived from the original variety and the chromosome derived from the foreign variety. Commonly used DNA markers can be used. The DNA marker may be, for example, a marker that can detect gene polymorphism such as SNP (Single Nucleotide Polymorphism, single gene polymorphism) or SSR (Simple Sequence Repeats, simple repeat sequence), and the like, and the like. An RFLP (Restriction Fragment Length Polymorphism) marker may also be used. In addition, discrimination between the original variety-derived alleles and the foreign variety-derived alleles by these DNA markers can be performed by a conventional method. For example, using DNA extracted from each individual as a template, performing PCR using a primer that can specifically hybridize with a specific SNP or SSR, detecting the presence or absence of a PCR product using electrophoresis or the like, Polymorphism can be identified. In addition, after DNA extracted from each individual is treated with a restriction enzyme, the pattern of the DNA fragment can be detected using electrophoresis or the like to identify each polymorphism. A primer that can specifically hybridize with a specific SNP or SSR can be designed by a conventional method using a commonly used primer design tool or the like according to the base sequence of the SNP or SSR. In addition, designed primers and the like can be synthesized using any method well known in the art.

  As these DNA markers, known DNA markers can be appropriately used. Moreover, the DNA marker produced newly may be sufficient. As known DNA markers, for example, in rice, the SNP marker disclosed in International Publication No. 2003/070934, etc., Rice Genome Research Program (RGP: http://rgp.dna.affrc.go.jp.jp) /Publicdata.html) publicly available DNA markers can be used.

  The gene information and the like of each variety can be obtained from, for example, NCBI (National Center for Biotechnology Information) and DDBJ (DNA Data Bank of Japan) which are international base sequence databases. In particular, genetic information of rice varieties can be obtained at KOME (Knowledge-based Oryzal Molecular Biological Encyclopedia, http://cdna01.dna.affrc.go.jp/cDNA/) and the like.

  In the present invention and the specification of the present application, “region from the Xth base to the Yth base of the chromosome of rice cultivar Nipponbare” is the nucleotide sequence (version 4; IRGSP- This is an area determined on the basis of build4-06 / 04/21).

  Further, in the present invention and the present specification, “the region corresponding to the region from the Xth base to the Yth base of the chromosome of rice cultivar Nipponbare” refers to the chromosome of the rice cultivar Nipponbare in the chromosome of the rice individual. This region is highly homologous to the region, and can be determined by aligning the known genomic DNA of the rice cultivar Nipponbare and the base sequence of the genomic DNA of the rice individual so as to have the highest homology. In addition, “SNPs corresponding to SNPs of rice varieties Nipponbare” in rice individuals other than rice varieties Nipponbare include the known genomic DNA of rice varieties Nipponbare and the genomic DNA of the rice individual in the region containing the SNP. , When aligned so that the homology is highest, it means a base at a position corresponding to the SNP.

  In order to breed new varieties that can be cultivated in a region north of conventional varieties, the inventors of the present invention first crossed rice varieties Habataki and rice varieties Koshihikari with respect to the heading period, and QTL ( Quantitative Trait Locus) analysis was performed. As a result, the QTS14 region of the long arm of chromosome 3 of rice cultivar Habataki [region corresponding to the region from the 31st, 720, 064th base to the 31st, 724, 043th base of the 3rd chromosome of rice cultivar Nipponbare] It was also found that there is a QTL for early heading and early birth. Therefore, the present inventor has produced a new variety in which a gene contained in the region of Koshihikari is replaced with a gene derived from Habataki. The new variety was expected to be an earlier rice than the original variety Koshihikari.

  When plant varieties are improved by non-genetical recombination methods, if the introduced chromosomal fragment is too large, many other genes with unknown functions other than the target trait gene may be introduced. There is a risk of damaging the favorable traits of the original variety. Therefore, in order to produce a new variety having a target trait without changing the preferable trait of the original cultivar, the present inventor controls the substitution region by the chromosome fragment derived from the introduced foreign cultivar. New varieties were produced by the method described.

  The method for producing a new variety described in Patent Document 2 is specifically as follows. First, five types of DNA markers having a positional relationship as shown in FIG. 1 were set based on known rice gene information. That is, the DNA marker M2 is upstream of the target region T or upstream thereof, the DNA marker M1 is upstream of the DNA marker M2, the DNA marker M4 is downstream of the target region T or downstream thereof, and the DNA marker M4 is downstream. DNA marker M5 is set in the target region T, and DNA marker M3 is set in the target region T. Next, backcrossing is performed on a chromosome fragment-substituted strain in which only a part of the Koshihikari chromosome including the target region T is replaced with a Habataki-derived chromosome fragment, and the above five kinds of DNA are obtained from the obtained hybrid population. A preferable individual is selected based on the markers M1 to M5. Thereafter, self-mating or back-crossing is appropriately performed on the individual, and similarly, selecting a preferable individual based on the DNA markers M1 to M5 is repeated as appropriate, thereby upstream of the region replaced with the Habataki-derived chromosome fragment. A progeny individual having a side end between the DNA markers M1 and M2 and a downstream end of the region between the DNA markers M4 and M5 can be obtained. As shown in FIG. 1, in the progeny individuals, the DNA markers M1 and M5 are the same type as the original variety, and the DNA markers M2, M3, and M4 are the same type as the foreign variety (in the present invention, Habataki). .

  Here, in the method for producing a new variety described in Patent Document 2, if the distance d1 between the DNA markers M1 and M2 is long, the upstream end of the foreign-variety-derived chromosome fragment (in this application, Habataki-derived chromosome fragment) L exists. The range to be obtained is wide, and the length of the introduced Habataki-derived chromosome fragment L is difficult to determine. On the other hand, if the distance d1 is short, the range in which the upstream end of the Habataki-derived chromosome fragment L can exist is narrow, and the length of the Habataki-derived chromosome fragment L to be introduced is easily determined. Similarly, if the distance d3 between the DNA markers M4 and M5 is long, the range in which the downstream end of the Habataki-derived chromosome fragment L can exist is wide, and the length of the Habataki-derived chromosome fragment L to be introduced becomes difficult to determine. If d3 is short, the range in which the downstream end of Habataki-derived chromosome fragment L can exist is narrow, and the length of Habataki-derived chromosome fragment L to be introduced is easily determined.

  Specifically, the set of DNA markers M1 to M5 shown in Table 1, that is, the SNP corresponding to the 31st, 521st, and 442nd SNPs (single nucleotide polymorphisms) of the third chromosome of the rice variety Nipponbare (in the rice variety Koshihikari) A, C in the rice cultivar Habataki is the DNA marker M1 (DNA marker M1-Ac (QTS14)), and the SNP corresponding to the 31st, 689th, and 690th SNPs of chromosome 3 of the rice cultivar Nipponbare (C in the rice cultivar Koshihikari is C In the rice cultivar Habataki, T) is the DNA marker M2 (DNA marker M2-Ct (QTS14)), and the SNP corresponding to the 32,208,924th SNP of chromosome 3 of the rice cultivar Nipponbare is A (in rice cultivar Koshihikari, A, In rice varieties Habataki, G) is the DNA marker M3 (DNA marker M3-Ag (QTS14)). The SNP corresponding to the 32,298,686th SNP of chromosome 3 of rice cultivar Nipponbare (G for rice cultivar Koshihikari and C for rice cultivar Habataki) is defined as DNA marker M4 (DNA marker M4-Gc (QTS14)). The SNP corresponding to the 32,363,157th SNP of chromosome 3 of cultivar Nipponbare (A for rice cultivar Koshihikari and T for rice cultivar Habataki) was used as DNA marker M5 (DNA marker M5-At (QTS14)). A new variety was produced by the method for producing a new variety described in Patent Document 2. From these results, the region from the DNA marker M2-Ct (QTS14) to the DNA marker M4-Gc (QTS14) in the third chromosome of the rice individual (that is, 31,689, A new cultivar was produced in which the region including the region from the 690th base to the 32,298,686th base) was replaced with a Habataki-derived chromosome fragment. In the new variety, the upstream end of the Habataki-derived chromosome fragment is located downstream from the DNA marker M1-Ac (QTS14) and up to the DNA marker M2-Ct (QTS14) (that is, the third chromosome of the rice variety Nipponbare). In the region from the 31st, 521, 443rd base to the 31st, 689th, 690th base), and the downstream end of the chromosome fragment is from the DNA marker M4-Gc (QTS14) to the DNA marker A region upstream from M5-At (QTS14) (ie, a region corresponding to the region from the 32,298,686th base to the 32,363,156th base in the third chromosome of rice cultivar Nipponbare) Exists.

  The present inventor has named this new variety “Koshihikari Eichi No. 5”. FIG. 2 is a diagram schematically showing the genomes of Koshihikari and Koshihikari eichi No.5. In the field in Chiba Prefecture, the heading time of Koshihikari eichi No. 5 was measured (seeding date: May 6, 2010, transplanting date: June 1, 2010). As shown in FIG. The heading period was from August 5 to August 8, whereas Koshihikari Eichi No. 5 was from July 24 to July 26. In other words, Koshihikari Eichi No. 5 was clearly found to be early born compared to the original variety Koshihikari.

  Furthermore, the heading time of Koshihikari Eichi No. 5 was measured in a field in Hokkaido north of 38.5 degrees north latitude (seeding date: April 28, 2010, transplanting date: June 7, 2010). As a result, as shown in FIG. 4, the heading period of Koshihikari was from September 1 to September 2, whereas Koshihikari Eichi No. 5 was from August 21 to August 22. . In other words, even when cultivated in Hokkaido, Koshihikari Eichi No. 5 was clearly found to be early growing compared to the original variety Koshihikari. However, although Koshihikari and Koshihikari eichi No. 5 both headed, they did not mature sufficiently and could not harvest rice.

  The inventor of the present invention may be able to obtain Koshihikari that is early enough to be cultivated even in the northern region by stacking foreign chromosome fragments having an early-emergence function on Koshihikari eichi-5. Thought. Therefore, Koshihikari Eichi No. 5 and the rice variety Koshihikari Eichi No. 3 were crossed.

  Koshihikari eichi 3 is a variety in which only the region containing the Hd1 gene of chromosome 6 in Koshihikari's chromosome is replaced with a gene fragment derived from Habataki by the method for producing a new variety described in Patent Document 2. Table 2 shows five types of DNA markers used for the production of Koshihikari eichi 3go. DNA marker M1-Ct is a SNP corresponding to the 8th, 757, and 818th SNP of chromosome 6 of rice cultivar Nipponbare (C for rice cultivar Koshihikari and T for rice cultivar Habataki), and DNA marker M2-Ag is The SNP corresponding to the 8,940,503rd SNP of chromosome 6 of rice cultivar Nipponbare (A in rice cultivar Koshihikari, G in rice cultivar Habataki), and DNA marker M3-Cg is chromosome 6 of rice cultivar Nipponbare SNP (C for rice cultivar Koshihikari and G for rice cultivar Habataki), and DNA marker M4-Gc is the 9th, 533, 057th chromosome 6 of rice cultivar Nipponbare SNP (G for rice cultivar Koshihikari, C for rice cultivar Habataki), and DNA marker M5 At is a SNP corresponding to 9,777,196 th SNP of chromosome 6 of rice cultivar Nipponbare (rice varieties Koshihikari A, T is a rice cultivar Habataki). That is, Koshihikari eichi 3 is a region from the DNA marker M2-Ag (Hd1) to the DNA marker M4-Gc (Hd1) in the chromosome 6 of the rice variety Koshihikari (that is, in the chromosome 6 of the rice variety Nipponbare). A region including the region from the 8,940,503rd base to the 9,533,057th base) is a new variety in which a Habataki-derived chromosome fragment is replaced. In the new variety, the upstream end of the Habataki-derived chromosome fragment is located downstream from the DNA marker M1-Ct (Hd1) and up to the DNA marker M2-Ag (Hd1) (that is, chromosome 6 of the rice variety Koshihikari). The region from the 8,757,819th base to the 8,940,503th base), and the downstream end of the chromosomal fragment is from the DNA marker M4-Gc (Hd1) to the DNA marker. It exists in a region upstream of M5-At (Hd1) (that is, a region corresponding to a region including the 9,533,057th base to the 9,777,195th base).

  FIG. 5 is a diagram schematically showing the genomes of Koshihikari and Koshihikari eichi 3go. In a field in Chiba Prefecture, the heading time of Koshihikari eichi 3 was measured (seeding date: May 6, 2010, transplanting date: June 1, 2010). As shown in FIG. The heading period was from August 5 to August 8, whereas Koshihikari Eichi 3 was from July 25 to July 26. In other words, when cultivated in Chiba Prefecture, Koshihikari Eichi 3 was as early as Koshihikari Eichi 5.

  Furthermore, the heading time of Koshihikari Eichi 3 was measured in a field in Hokkaido north of 38.5 degrees north latitude (seeding date: April 28, 2010, transplanting date: June 7, 2010). As a result, as shown in FIG. 7, the heading time of Koshihikari was from September 1 to September 2, and rice could not be harvested. On the other hand, the heading time of Koshihikari Eichi 3 was from August 10 to August 16, and rice could be harvested thereafter. In other words, Koshihikari Eichi No. 3 grows significantly faster than Koshihikari Eichi No. 5 when cultivated in a region north of 38.5 degrees north latitude, so it can be cultivated in Hokkaido. It became clear. The degree of early-proliferation effect by replacing the Hd1 region with Habataki-derived chromosomal fragments varies depending on the cultivated place, for example, when cultivated in a northern region, for example, a region north of latitude 38.5 degrees north. It is a finding for the first time by the present inventor that the effect of fast-growing is higher than when cultivated in the Koshihikari cultivation area (35.5 to 38.5 degrees north latitude).

  As shown in Example 1 below, the present inventor crossed Koshihikari eichi 5 and Koshihikari eichi 3 and only the QTS14 region and the Hd1 region were replaced with habataki-derived chromosome fragments in the Koshihikari chromosome. New varieties were made. The inventor named this new variety “Koshihikari Kazusa No. 6”. FIG. 8 is a diagram schematically showing the genome of Koshihikari Kazusa No. 6. When the heading time of Koshihikari Kazusa No. 6 was measured, it was earlier than Koshihikari Eichi No. 3, and even when cultivated in Hokkaido north of 38.5 degrees north latitude, rice could be harvested. Moreover, when the expression character of Koshihikari Kazusa No. 6 was compared with Koshihikari, in the actual field test, other characters other than the heading time were almost the same as Koshihikari.

Koshihikari Kazusa No. 6 is a new variety produced by the method described in Patent Document 2, and has been designed and cultivated such that 99% or more of the genome structure is the same as Koshihikari. Koshihikari Kazusa No. 6 is a very good variety that maintains excellent traits such as the taste of Koshihikari despite being so fast that it can be cultivated in Hokkaido, where Koshihikari could not be cultivated. . Therefore, the applicant has deposited Koshihikari Kazusa No. 6 as a new plant at the National Institute of Advanced Industrial Science and Technology Patent Biological Deposit Center (1-1-1 Tsukuba Center, Tsukuba City, Ibaraki Prefecture) (Deposit Date: September 20, 2011). The accession number is FERM P- 22175.

  Rice cultivar Koshihikari Kazusa No. 6 can be cultivated by the same method as the original cultivar Koshihikari, and rice can be harvested by self-mating or artificial mating. In addition, the rice variety Koshihikari Kazusa No. 6 and its progeny individuals can be used as parent individuals for breeding new varieties, similar to the original variety Koshihikari. For example, trying to breed a new variety by crossing an individual of the rice variety Koshihikari Kazusa No. 6 with an individual of another variety and backcrossing the obtained progeny individual with an individual of the rice variety Koshihikari Kazusa No. 6 You can also.

  Further, the five types of DNA markers shown in Table 1 (DNA marker M1-Ac (QTS14), DNA marker M2-Ct (QTS14), DNA marker M3-Ag (QTS14), DNA marker M4-Gc (QTS14) are: Genome information unique to rice cultivar Koshihikari Kazusa No. 6 and rice cultivar Koshihikari Kazuichi 5. Therefore, rice cultivar Koshihikari Kazusa 6 and rice cultivar Koshihikari Kazuichi 5 use these five kinds of DNA markers as appropriate. Can be distinguished.

  Specifically, genome analysis is performed on rice individuals to be cultivated, and DNA markers M1-Ac (QTS14), DNA markers M2-Ct (QTS14), DNA markers M3-Ag (QTS14), DNA markers One or more DNA markers selected from the group consisting of M4-Gc (QTS14) and DNA marker M5-At (QTS14) are typed, and the obtained typing results are consistent with the results of rice cultivar Koshihikari Kazusa No. 6 In this case, the rice individual can be identified as the rice variety Koshihikari kazusa No. 6 or the rice variety Koshihikari eichi No. 5.

  In addition, five types of DNA markers shown in Table 2 (DNA marker M1-Ct (Hd1), DNA marker M2-Ag (Hd1), DNA marker M3-Cg (Hd1), DNA marker M4-Gc (Hd1), and The DNA marker M5-At (Hd1)) is genomic information unique to the rice cultivar Koshihikari Kazusa No. 6 and the rice cultivar Koshihikari eichi 3go. Therefore, the rice cultivar Koshihikari kazusa No. 6 and the rice cultivar Koshihikari eichi 3 can be distinguished using these five types of DNA markers as appropriate.

  Specifically, genome analysis is performed on rice individuals to be cultivated, and DNA markers M1-Ct (Hd1), DNA markers M2-Ag (Hd1), DNA markers M3-Cg (Hd1), DNA markers One or more DNA markers selected from the group consisting of M4-Gc (Hd1) and DNA marker M5-At (Hd1) are typed, and the obtained typing result is consistent with the result of rice cultivar Koshihikari Kazusa No. 6 In this case, the rice individual can be identified as the rice variety Koshihikari kazusa No. 6 or the rice variety Koshihikari eichi No. 3.

  Here, for discrimination of cultivars, all of the DNA markers M1 to M5 may be used, or some of the five DNA markers may be used. For example, only DNA markers M1 and M2 that are upstream recombination points may be used, only DNA markers M4 and M5 that are downstream recombination points may be used, or only DNA markers M2 and M4 may be used. Good. By appropriately combining a plurality of DNA markers, more rigorous product identification becomes possible.

  From these results, the QTS14 region in the third chromosome of rice individuals, specifically, the region from at least the DNA marker M2-Ct (QTS14) to the DNA marker M4-Gc (QTS14) (that is, the rice cultivar Nipponbare No. By substituting a region corresponding to the region from the 31st, 689th and 690th bases to the 32nd, 298th and 686th bases in 3 chromosomes with a chromosomal fragment of the rice cultivar Habataki. It is clear that individuals can be born faster than the original variety. The region of rice cultivar Koshihikari kazusa 6 and rice cultivar Koshihikari eichi 5 is composed of a chromosome fragment comprising the region of rice cultivar Habataki, so rice cultivar Koshihikari kazusa 6 or rice cultivar Koshihikari eichi You may substitute by the chromosome fragment which consists of the said area | region of No. 5. A rice individual that is rapidly grown by introducing a chromosome fragment of the region of the rice variety Habataki may be any variety that has the same or similar base sequence as the rice variety Koshihikari. Although it is not limited, it is preferable that it is a rice variety Koshihikari or a new variety produced as a parent variety from the viewpoint of consumer preference.

  The upstream end of the chromosome fragment derived from rice cultivar Habataki (or derived from rice cultivar Koshihikari Kazusa No. 6 etc.) including the region from DNA marker M2-Ct (QTS14) to DNA marker M4-Gc (QTS14) is the DNA marker M1. -The region downstream of Ac (QTS14) and up to the DNA marker M2-Ct (QTS14) (ie, the 31st, 689th, and 690th bases from the 31st, 521st, and 443rd bases in the third chromosome of the rice cultivar Nipponbare In which the downstream end of the chromosome fragment is located upstream from the DNA marker M4-Gc (QTS14) to the DNA marker M5-At (QTS14) (ie, rice cultivar) Number 32,363,156 from the 32,298,686th base in the third chromosome of Nipponbare In the region containing up to the base of the rice) by introducing the chromosome fragment into the third chromosome of the rice individual, without apparently affecting the traits other than the heading stage. Individuals can be born faster than the original variety.

  In addition to the QTS14 region in the third chromosome, the Hd1 region in the sixth chromosome, specifically, the region from at least the DNA marker M2-Ag (Hd1) to the DNA marker M4-Gc (Hd1) (ie, , The region corresponding to the region from the 8,940,503th base to the 9,533,057th base in the 6th chromosome of the rice cultivar Nipponbare) is replaced with a chromosomal fragment comprising this region of the rice cultivar Habataki By doing so, the rice individual can be remarkably fastened so that it can be cultivated in a region north of 38.5 degrees north latitude. The region of the rice cultivar Koshihikari Kazusa 6 and the rice cultivar Koshihikari eichi 3 is composed of a chromosome fragment comprising the region of the rice cultivar Habataki. You may substitute by the chromosome fragment which consists of the said area | region of No. 3. A rice individual that is rapidly grown by introducing a chromosome fragment of the region of the rice variety Habataki may be any variety that has the same or similar base sequence as the rice variety Koshihikari. Although it is not limited, it is preferable that it is a rice variety Koshihikari or a new variety produced as a parent variety from the viewpoint of consumer preference.

  Further, the upstream end of the chromosome fragment derived from rice cultivar Habataki (or from rice cultivar Koshihikari Kazusa No. 6 etc.) including the region from the DNA marker M2-Ag (Hd1) to the DNA marker M4-Gc (Hd1) is the DNA marker M1. -The region downstream of Ct (Hd1) and up to the DNA marker M2-Ag (Hd1) (ie, from the 8,757,819th base in the chromosome 6 of the rice cultivar Nipponbare to the 8,940,503th base) In which the downstream end of the chromosome fragment extends from the DNA marker M4-Gc (Hd1) to the upstream of the DNA marker M5-At (Hd1) (ie, rice cultivar). Corresponds to the region that includes the 9,533,057th base to the 9,777,195th base in Nipponbare chromosome 6. By introducing the chromosome fragment into the 6th chromosome of a rice individual so that it exists in the area), the rice individual can be made faster than the original cultivar without apparently affecting the traits other than the heading stage. can do.

  The Hd1 region in chromosome 6, including Koshihikari eichi 3 and Koshihikari kazusa 6 (specifically, at least from DNA marker M2-Ag (Hd1) to DNA marker M4-Gc (Hd1)) The rice plant whose region is replaced with a chromosome fragment comprising the region of the rice variety Habataki is not only cultivatable in areas where Koshihikari can be cultivated, but also cultivated in areas north of latitude 38.5 degrees north, Rice can be harvested. These rice individuals are affected by temperature, rainfall, and the like, but can be cultivated in an area between 38.5 degrees and 43.3 degrees north latitude, for example.

  From the studies so far, it is considered that the Hd1 gene in the Hd1 region is a causative gene causing premature growth. On the other hand, when a gene contained in the QTS14 region was examined, a region encoding the phytochrome C gene was included in the region. It has been reported that this gene is mainly involved in the control of plant flowering time (US Pat. No. 7,656,815). Therefore, it is inferred that the causative gene causing prematurity in the QTS14 region is the phytochrome C gene. In the allele fragment of the rice cultivar Nipponbare, the Hd1 gene is mapped to the region from the 9,335,337th base to the 9,337,606th base of chromosome 6, and the phytochrome C gene is Maps to the region from the 31st, 720, 064th base to the 31st, 724, 043th base of the 3 chromosome.

  It is shorter than the Habataki-derived chromosome fragment introduced in Koshihikari Kazusa No. 6 if the region containing the early-causing gene in the Hd1 region or the region containing the early-causing gene in the QTS14 region is replaced by a Habataki-derived chromosome fragment Even in rice individuals that have been replaced by chromosome fragments, it is thought that premature growth is caused, as in the rice cultivar Koshihikari Kazusa No. 6. Therefore, for example, the region corresponding to the region from the 31st, 689th, 691st base to the 31st, 724th, 043th base in the 3rd chromosome of the rice variety Nipponbare in the 3rd chromosome of the rice individual It is considered that the rice individual can be born faster than the original cultivar by substituting the cultivar Koshihikari Kazusa No. 6, the rice cultivar Koshihikari eichi No. 5 or the rice cultivar Habataki with the chromosome fragment. At this time, the upstream end of the chromosome fragment is present in a region corresponding to the region from the 31st, 689th, 690th base to the 31st, 720, 064th base of the third chromosome of the rice cultivar Nipponbare, And the chromosome fragment so that the downstream end of the chromosome fragment exists in a region corresponding to the region from the 31st, 724, 043th base to the 32,298, 685th base of the third chromosome of rice cultivar Nipponbare. By introducing a fragment into the third chromosome of a rice individual, it is considered that the rice individual can be made faster than the original variety without clearly affecting the traits other than the heading stage.

  Similarly, the region corresponding to the region from the 9,335,337th base to the 9,337,606th base in the 6th chromosome of the rice variety Nipponbare in the 6th chromosome of the rice individual, By replacing the Koshihikari kazusa No. 6, the rice cultivar Koshihikari eichi 3 or the rice cultivar Habataki with a chromosomal fragment, it is considered that the rice individual can be born faster than the original cultivar. At this time, the upstream end of the chromosome fragment is present in a region corresponding to a region including the bases from the 8,940,504th base to the 9,335,337th base of the sixth chromosome of the rice cultivar Nipponbare, And the chromosome fragment so that the downstream end of the chromosome fragment exists in a region corresponding to the region from the 9,337,606th base to the 9,533,056th base of the third chromosome of rice cultivar Nipponbare. By introducing a fragment into the third chromosome of a rice individual, it is considered that the rice individual can be made faster than the original variety without clearly affecting the traits other than the heading stage.

  EXAMPLES Next, although an Example is shown and this invention is demonstrated further in detail, this invention is not limited to a following example.

[Example 1]
Koshihikari Eichi No. 5 and Koshihikari Eichi No. 3 were crossed to produce a new variety in which only the QTS14 region and the Hd1 region were replaced with Habataki-derived chromosome fragments in the Koshihikari chromosome.
Specifically, Koshihikari eichi 3 and Koshihikari eichi 5 are crossed, 2 of the obtained progeny individuals (seed) are cultivated, self-propagated (self-mating), and seeds that are progeny individuals 100 pieces were obtained. All 100 seeds are cultivated, the DNA markers of each progeny individual are examined, and the cultivated individuals in which both DNA marker M3-Cg (Hd1) and DNA marker M3-Ag (QTS14) are homochromosomal regions of the Habataki allele One individual was selected. The inventor named this new variety “Koshihikari Kazusa No. 6”.

  The heading time of Koshihikari Kazusa No. 6 was measured in a field in Chiba Prefecture (seeding date: May 6, 2010, transplanting date: June 1, 2010). The measurement results are shown in FIG. 9 together with the results of Koshihikari, Koshihikari eichi 5 and Koshihikari eichi 3. Koshihikari's heading date is from August 5 to August 8, and Koshihikari Eichi 5 and Koshihikari Eichi 3 are from July 24 to July 26, while Koshihikari Kazusa 6 Was from July 18th to July 23rd. From these results, when cultivated in Chiba Prefecture, Koshihikari Kazusa No. 6 was clearly earlier than Koshihikari Eichi No. 3 and Koshihikari Echigo No. 5.

  Furthermore, the heading time of Koshihikari Kazusa No. 6 was measured in a farm field in Hokkaido (43.3 degrees north latitude) (seeding date: April 28, 2010, transplanting date: June 7, 2010). The measurement results are shown in FIG. 10 together with the results of Koshihikari, Koshihikari eichi 5 and Koshihikari eichi 3. Koshihikari's heading date is from September 1 to September 2, Koshihikari Eichi No. 5 is from August 21 to August 22, and Koshihikari Eichi No. 3 is from August 10 to August 16. In contrast, Koshihikari Kazusa No. 6 was from August 7th to August 9th. Moreover, Koshihikari and Koshihikari eichi No. 5 did not mature, while Koshihikari kazusa No. 6 was able to harvest rice in the same manner as Koshihikari eichi no. 3. From these results, it is clear that Koshihikari Kazusa No. 6 can be cultivated in Hokkaido north of 38.5 degrees north latitude.

  The characteristics of Koshihikari Kazusa No. 6 and Koshihikari were compared (implemented in Chiba Prefecture in 2009). The examination of the traits was conducted in accordance with the characteristic examination for the variety registration application based on Article 5 Paragraph 1 of the Seedling and Seedling Law (Act No. 83 of 1998). The examination results are shown in Tables 3-6. As a result, Koshihikari Kazusa No. 6 was about two weeks ahead of Koshihikari in both heading and maturity. Koshihikari Kazusa No.6 was slightly shorter than the Koshihikari, but the stem length and main stem length and main stem length were slightly shorter, and the number of ears and the number of main stem grains were smaller, but other traits were basically Koshihikari. Was the same.

  The rice cultivar Koshihikari Kazusa No. 6 which is a new variety of the present invention has almost the same characteristics as Koshihikari, and can be cultivated in the northern region more than before, so it can be used particularly in the field of agriculture. Moreover, since the rice individual of the present invention can be made to grow faster than the original variety, the method can be used particularly in the field of plant breeding.

FERM P- 22175

Claims (2)

Rice cultivar Koshihikari Kazusa No. 6 with an accession number of FERM P- 22175 (Oryza sativa L. multivar Koshihikari-kazusa6 gou).   A progeny individual obtained by mating two individuals selected from the group consisting of an individual of the variety according to claim 1 and a progeny individual of the individual of claim 1.

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