Allele-Dependent Barley Grain beta -Amylase Activity

doi:10.1104/pp.117.2.679

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Allele-Dependent Barley Grain $beta$ -Amylase Activity¹

Maria J. Erkkilä², Robert Leah, Hannu Ahokas, and Verena Cameron-Mills^*

Carlsberg Research Laboratory, Gamle Carlsberg Vej 10, DK-2500, Copenhagen, Denmark (M.J.E., R.L., V.C.-M.); and Plant Breeding Section, Agricultural Research Centre, FIN-31600 Jokioinen, Finland (H.A.)

ABSTRACT

Top
Abstract
Introduction
Methods
Results
Discussion
References

The wild ancestor of cultivated barley, Hordeum vulgare subsp. spontaneum (K. Koch) A. & Gr. (H. spontaneum), is a sourceof wide genetic diversity, including traits that are importantfor malting quality. A high $beta$ -amylase trait was previously identifiedin H. spontaneum strains from Israel, and transferred into thebackcross progeny of a cross with the domesticated barley cv Adorra.We have used Southern-blot analysis and $beta$ -amy1 gene characterizationto demonstrate that the high $beta$ -amylase trait in the backcrossline is co-inherited with the $beta$ -amy1 gene from the H. spontaneumparent. We have analyzed the $beta$ -amy1 gene organization in variousdomesticated and wild-type barley strains and identified threedistinct $beta$ -amy1 alleles. Two of these $beta$ -amy1 alleles were presentin modern barley, one of which was specifically found in goodmalting barley cultivars. The third allele, linked with high grain $beta$ -amylase activity, was found only in a H. spontaneum strain fromthe Judean foothills in Israel. The sequences of three isolated $beta$ -amy1 alleles are compared. The involvement of specific intronIII sequences, in particular a 126-bp palindromic insertion, inthe allele-dependent expression of $beta$ -amylase activity in barleygrain is proposed.

INTRODUCTION

Top
Abstract
Introduction
Methods
Results
Discussion
References

The endosperm of barley (Hordeum vulgare L.) and other cereals is a storage organ in which starch and protein accumulate duringgrain development and are later degraded to provide energy andN₂ during germination and seedling growth (for review, see MacGregorand Fincher, 1993). Starch degradation in the cereal grain requiresthe concerted action of several enzymes (MacGregor, 1987), includinglimit dextrinase, $beta$ -amylase, $alpha$ -glucosidase (Sun and Henson, 1990),and $alpha$ -amylases. $beta$ -Amylase is a 1,4- $alpha$ -D-glucan maltohydrolase (EC3.2.1.2.), which catalyzes the liberation of maltose and limitdextrins from the nonreducing ends of starch (Robyt and Whelan,1968; Sopanen and Laurière, 1989).

$beta$ -Amylase is synthesized during grain development (Kreis et al., 1987) and is one of the major proteins found in the starchyendosperm (Hejgaard and Boisen, 1980). In dry barley grains itis found in two forms: a free, active form and a bound, less-activeform, the latter accounting for about 75% of the total $beta$ -amylase.Both forms may be aggregated or disulfide bonded via a Cys residuenear the C terminus to other grain proteins such as protein Z(Hejgaard, 1978). The free form of $beta$ -amylase is easily extractablein saline solutions and comprises many forms separable by IEF(Shewry et al., 1988). The release and activation of $beta$ -amylaseduring germination is accompanied by the accumulation of additional $beta$ -amylase isoforms (Sopanen and Laurière, 1989; Guerin et al.,1992), which could be caused by a progressive endoproteolyticremoval of C-terminal peptides (Lundgard and Svensson, 1987).

Synthesis of $beta$ -amylase during barley grain development is regulated by nutritional N₂ (Giese and Hopp, 1984), and high levelsof $beta$ -amylase are generally correlated with increased grain proteincontent (Santos and Riis, 1996). Modern plant breeding has reducedthe genetic variability among domesticated barley cultivars (Thompsonet al., 1990; Forster et al., 1991). This in turn limits the potentialfor selecting cultivars with high $beta$ -amylase levels independentof grain protein content, which is an important quality parameterfor malt barley. However, a large genetic diversity is found inH. vulgare subsp. spontaneum (K. Koch) A. & Gr. (abbreviated toH. spontaneum), the wild ancestor of cultivated barley (Wiberg,1974; Zhang et al., 1993; Saghai Maroof et al., 1995). H. spontaneumstrains from Israel and Jordan show a wide variation in $beta$ -amylase, $beta$ -glucanase, and other hydrolase activities (Ahokas and Naskali,1990a, 1990b). We have previously shown that a high $beta$ -amylasetrait in selected H. spontaneum strains is inherited in the backcrossedprogeny of H. spontaneum and domesticated barley (Ahokas and Erkkilä,1992), which may be linked to inheritance of a $beta$ -amy allele ofH. spontaneum.

To study the biochemical and molecular mechanisms underlying the different levels of $beta$ -amylase activity in domesticated barleyand its wild ancestors, we have isolated and characterized the $beta$ -amylase cDNAs and genes from the H. spontaneum × domesticatedbarley backcross and the respective parental lines generated byAhokas and Erkkilä (1992). We report here that the observed differencesin $beta$ -amylase activity in the grains are correlated with sequencedifferences in the $beta$ -amy1 gene, which involve the insertion/deletionof a palindromic 126-bp sequence and a 39-bp sequence in intronIII, as well as two amino acid substitutions in the ORF. We haveexploited the sequence variation in intron III to develop a PCRmethod to explore the genetic diversity of the $beta$ -amy1 locus amongdomesticated and wild barley and to develop a screening tool forbreeding lines with high $beta$ -amylase activity.

	MATERIALS AND METHODS

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Barley (Hordeum vulgare) plants were grown either in a greenhouse or in fields in the southern part of Finland. Grains ofvarious barley cultivars were provided by the Agricultural ResearchCentre of Finland (Jokioinen) and cv Haruna Nijo was providedby Sapporo Brewing, Ltd. (Yaizu, Japan). The grain material analyzedincluded BC-F₆ lines derived from a single backcross of Hordeumspontaneum × Adorra (accession no. PI 296897) from the U.S. Departmentof Agriculture (Beltsville, MD), followed by six generations ofselection for the domesticated growth habit, and the two parents(cv Adorra and H. spontaneum). An additional line, denoted strain86-H2-64, was selected in the sixth generation from an independentbut similar single backcross. The accession PI 296897 originatedfrom the Judean Foothills near Jerusalem, Israel. Other wild barleysused for testing $beta$ -amy1 allele diversity were H. spontaneum strainscollected from the Israeli localities of Talpiyyot, Mehola, Atlit,Negev, and from Cyprus, and Hordeum murinum subsp. leporinum fromCorsica (France).

Assays of $beta$ -Amylase Activity

$beta$ -Amylase activity and grain protein content were determined in grain samples (2 g) milled in an A/10 analytical mill (Jankeand Kunkel, Staufen, Germany). $beta$ -Amylase activity was assayedin duplicate samples of 0.5 g of fresh flour or 0.5 g of flourstored at $-$ 80°C using the Beta-Amylase Kit from Megazyme (Bray,Ireland), according to the method of Santoz and Riis (1996). Oneunit of $beta$ -amylase activity is defined as the amount of enzymerequired to release 1 µmol of p-nitrophenol from p-nitrophenyl- $alpha$ -D-maltopentaosein 1 min in the presence of excess $alpha$ -glucosidase under assay conditionsdefined in the kit. Total soluble protein in flour samples wasdetermined according to the method of Bradford (1976)

. $beta$ -Amylaseactivity values are expressed per milligram of protein in theflour.

RNA and DNA Protocols

Total RNA was extracted from endosperm tissue using aurintricarboxylic acid as the RNase inhibitor (Leah et al., 1991

) andfurther purified using the RNeasy Plant Total RNA kit (Qiagen,Chatsworth, CA).

DNA was extracted from 14-d-old leaves according to the method of Maniatis et al. (1982), or from 7-d-old leaves using FastPrep(BIO 101, Vista, CA) for PCR reactions. DNA sequencing was performed(model 373A sequencer, Applied Biosystems). The reaction mixturescontained 0.5 µg of DNA, 10 pmol of primer (20 bp), and the AmpliCycle Sequencing Kit (Perkin-Elmer). Sequences were analyzed withthe Micro Genie Sequence software package (Beckman).

Southern blotting and conditions for hybridizations were performed as described previously (Leah et al., 1991). Blots werehybridized with the 1750-bp $beta$ -amylase cDNA insert of pc $beta$ C51 (Kreiset al., 1987) labeled with [³²P]dCTP using the Megaprime DNA-labeling system (Amersham).

Allele-Specific $beta$ -Amy1 cDNA Cloning

cDNA was synthesized in two parts by RNA-PCR according to the method of Dyanov and Dzitoeva (1995)

with Moloney murine leukemiavirus reverse transcriptase (Boehringer Mannheim) from total RNAisolated from endosperm tissue (approximately 26 d after anthesis)of the different barley strains. The primers were based on thesequence of the $beta$ -amylase cDNA (Kreis et al., 1987

; Yoshigi etal., 1994

) or the cv Haruna Nijo $beta$ -amy gene (Yoshigi et al., 1995

The antisense primer for synthesis of the 5 $'$ part of the transcript was 5 $'$ -AGCAGATGAATTCTCCGATGCCTGGGAACGACC-3 $'$ , having anEcoRI site, together with the sense primer 5 $'$ -TAGCCAGGATCCACAATGGAGGTGAACGTGAAAGGC-3 $'$ ,having a BamHI site. The antisense primer for the 3 $'$ part of thetranscript was 5 $'$ -TAAACTCGAGGTTCCATTACATGGTGGCAGGGA-3 $'$ , havingan XhoI site, together with the sense primer 5 $'$ -CCCAGGCATCGGAGAATTCATCTGCTATGA-3 $'$ ,having an EcoRI site. The resulting PCR fragments were restrictedwith EcoRI, BamHI, and XhoI, purified, and ligated into pBluescriptSK vector (Stratagene) to produce full-length cDNA clones.

PCR Cloning of $beta$ -Amy1 Alleles

The promoter and ORF regions of the $beta$ -amy1 gene were amplified from genomic DNA of different barley strains using theExpand High-Fidelity PCR system (Boehringer Mannheim), accordingto the manufacturer's instructions. The PCR primers, based onthe sequence of the cv Haruna Nijo $beta$ -amy gene (Yoshigi et al.,1995

; EMBL accession nos. D63574 and D49999), were as follows:5 $'$ -ATTGGATCCATGGAGGTGAACGTGAAAGGCAACTATGTC-3 $'$ and 5 $'$ -AAAGGATCCATTACATGGTGGCAGGGAGCTCCCCACCCA-3 $'$ ,both with a 5 $'$ BamHI restriction site, for amplification of thegene ORF; and 5 $'$ -ACGCGTCGACACATCATCTTGAGAACGTCTTCTC-3 $'$ and 5 $'$ -ACGCGTCGACTCGAACCTGTTGTTCACGCTCAC-3 $'$ ,both with a 5 $'$ SalI restriction site, for amplification of thecorresponding promoter region.

The PCR reactions were performed as follows: DNA was denatured for 5 min at 95°C, followed by 30 cycles of 0.5 min at 94°C,1 min at 61°C, 3 min at 72°C, the last 20 cycles with a 20-s increasein extension time in each cycle, ending with a final polymerizationstep of 10 min at 72°C. The PCR fragments were cloned into pBluescriptSK vector (Stratagene).

$beta$ -amy1 intron III-specific sequences were amplified by PCR from genomic DNA of different barley lines with the following primerpair: 5 $'$ -GATGGTCGTTCCCAGGCATC-3 $'$ and 5 $'$ -AGGGAACCGCACGTGTGGGGTCAATGA-3 $'$ .The reaction mixture contained 0.5 to 0.7 µg of template DNA,10 pmol of each PCR primer, 0.2 mmol/L deoxyribonucleotide triphosphate,1.5 mmol/L MgCl₂, 50 mmol/L KCl, 10 mmol/L Tris-HCl (pH 9.0),0.1% Triton, and 1 unit of Taq polymerase (Promega). The mixturewas reacted for 2 min at 95°C, then for 1 min at 94°C, for 0.5min at 60°C, and for 1 min at 72°C for 25 cycles, followed by10 min at 72°C. The PCR fragments were detected in 5% polyacrylamidegels.

	RESULTS

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Identification of Three Distinct $beta$ -Amy1 Alleles

The organization of the $beta$ -amy1 structural gene in different barley strains was analyzed by Southern-blot analysis. GenomicDNA isolated from cv Haruna Nijo, cv Adorra, H. spontaneum PI296897, and line 86-H2-64 was restricted with HindIII, NcoI, SalI,and SpeI and hybridized with the $beta$ -amy1 pc $beta$ C51 cDNA (Kreis etal., 1987

). The size of the hybridizing fragments for each restrictiondigest was not identical in the four strains. For example, ina HindIII restriction digest (Fig. 1) the hybridizing fragmentswere approximately 7.0 kb in cv Adorra (lane 1), approximately9.0 kb in line 86-H2-64 and H. spontaneum PI 296897 (lanes 2 and3), and approximately 6.0 kb in cv Haruna Nijo (lane 4). An additionalhybridizing HindIII fragment of an approximately 1.6-kb fragmentwas detected in all four barley strains. Most of the hybridizingfragment sizes in cv Haruna Nijo DNA, including the 1.6-kb HindIIIfragment, were consistent with the sequence of this $beta$ -amy1 gene(Yoshigi et al., 1995

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Figure 1. Southern-blot analysis of the $beta$ -amy1 structural gene in different barley cultivars. Barley genomic DNA was digested with HindIII,fractionated by agarose-gel electrophoresis, Southern blotted,and hybridized with $beta$ -amy1 pc $beta$ C51 cDNA probe. The genomic DNAswere from cv Adorra (lane 1), line 86-H2-64 (lane 2), H. spontaneumPI 296897 (lane 3), and cv Haruna Nijo (lane 4).

The $beta$ -amy1 pc $beta$ C51 cDNA hybridizes to two loci in the barley genome, designated Bmy1 and Bmy2, located on chromosomes 4 and2, respectively (Kreis et al., 1988). The authors assigned a stronglyhybridizing HindIII fragment of 6.9 kb in cv Betzes to Bmy1, whereasa weaker hybridizing 4.7-kb fragment was assigned to Bmy2. Underthe hybridization conditions used here, hybridizing restrictionfragments that might correspond to the Bmy2 locus were not detected.In agreement with Kreis et al. (1988), restriction fragment lengthpolymorphism was observed at the Bmy1 locus, indicating the presenceof at least three distinct alleles in cv Haruna Nijo, cv Adorra,and H. spontaneum PI 296897. Furthermore, the strain 86-H2-64,derived from a H. spontaneum PI 296897 × Adorra cross and identifiedas having a high grain $beta$ -amylase activity, is seen to have inheritedthe H. spontaneum PI 296897-like $beta$ -amy1 allele.

Isolation and Characterization of the $beta$ -Amy1 Alleles and Their Transcripts

To identify the molecular mechanisms underlying the enhanced $beta$ -amylase activity in grain of H. spontaneum PI 296897 and itscv Adorra backcross progeny line 86-H2-64, we isolated and sequencedthe $beta$ -amy1 genes and transcripts from line 86-H2-64 and its parents.All three $beta$ -amy1 genes were PCR amplified from genomic DNA usingprimers based on the sequence of the $beta$ -amy1 gene from cv HarunaNijo, which is expressed in developing endosperm (Yoshigi et al.,1994

, 1995

). Single $beta$ -amy1 amplification products were generatedfrom each of the three barley strains and their sequences weredetermined. All four $beta$ -amy1 sequences were approximately 5 kbin length, comprising an ORF interrupted by six introns, as shownschematically in Figure 2, top. The sequences of the $beta$ -amy1 genesin line 86-H2-64 and H. spontaneum PI 296897 showed complete identity.The H. spontaneum PI 296897 $beta$ -amy1 allele showed high homologyto the $beta$ -amy1 allele of cv Haruna Nijo. Apart from a few single-basesubstitutions, sequence differences in cv Haruna Nijo $beta$ -amy1 wererestricted to the 5 $'$ -proximal end of intron III and a 25-bp deletionpositioned 761 bp upstream of the TATAA box. The cv Adorra $beta$ -amy1allele contained this upstream 25-bp insertion, and in additionto a number of single-base substitutions, showed significant sequencedivergence from H. spontaneum PI 296897 $beta$ -amy1, confined to intronIII.

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Figure 2. The $beta$ -amy1 gene organization. Top, Schematic presentation of the $beta$ -amy structural gene. The $beta$ -amy1 ORF is composed of sevenexons (black boxes) interrupted by six introns (numerals I-VI)located within a DNA fragment of approximately 5 kb. ATG, TAG,and gray box indicate the translational start and stop codonsand the approximately 1.3-kb promoter, respectively. Bottom, Sequencealignment of the 5 $'$ -proximal ends of intron III from $beta$ -amy1 allelesof H. spontaneum PI 296897 (2), cv Adorra (3), and cv Haruna Nijo(4). Line 1 shows the amino acid sequence (residues 195-205) encodedby the DNA sequence upstream of intron III. The sequences of intronIII from the $beta$ -amy1 allele of line 86-H2-64 (not shown) and H.spontaneum PI 296897 (2) are identical. The $beta$ -amy1 genomic sequencesare in the EMBL-GenBank database under accession numbers AF061204(H. spontaneum PI 296897), AF061203 (cv Adorra), and D49999(cv Haruna Nijo).

The cDNAs of the corresponding $beta$ -amy1 transcripts were cloned by reverse-transcriptase RNA-PCR. The sequences of the $beta$ -amy1cDNAs of H. spontaneum PI 296897, line 86-H2-64, and cv HarunaNijo were identical, apart from two silent nucleotide substitutionsin the latter. Four of the single-base substitutions found inthe cv Adorra $beta$ -amy1 allele were located in the ORF of the transcript.Two of these led to amino acid substitutions, namely Ala-233 $right-arrow$ Valand Ser-347 $right-arrow$ Leu, which are also seen in the cv Hiproly $beta$ -amy1allele (Kreis et al., 1987).

The major sequence differences between the three $beta$ -amy1 alleles were limited to the first 320 bp at the 5 $'$ end of intron III(Fig. 2, bottom). Compared with the published sequence of cv HarunaNijo, cv Adorra had a 126-bp insertion (Fig. 2, line 4 versusline 3), and H. spontaneum PI 296897 (and line 86-H2-64; datanot shown) had a 39-bp deletion (Fig. 2, line 4 versus line 2).

Inheritance of the H. spontaneum PI 296897-Like $beta$ -Amy1 Allele Is Linked to Enhanced $beta$ -Amylase Activity

We have shown that the high- $beta$ -amylase-activity trait in line 86-H2-64, an offspring of an H. spontaneum and domesticated barleycross (Ahokas and Erkkilä, 1992

), is linked to the inheritanceof the $beta$ -amy1 allele from H. spontaneum. To gain further evidencefor a close correlation between the H. spontaneum $beta$ -amy1 alleleand high $beta$ -amylase activity levels, we have studied a populationof 15 individual BC-F₆ lines from a H. spontaneum PI 296897 ×Adorra backcross grown under identical conditions. The two parental $beta$ -amy1 alleles inherited in the individual BC-F₆ lines were distinguishedby the allele-specific sequence of the $beta$ -amy1 intron III (Fig.2). This was accomplished by the design and use of PCR primersto amplify a region of the $beta$ -amy1 intron III, so that the cv Adorraallele was identified by a 643-bp PCR fragment, whereas the H.spontaneum PI 296897 allele was identified by a 477-bp PCR fragment(Fig. 3). Three of the offspring had inherited the H. spontaneumPI 296897 allele (Fig. 3, lane 2 versus lanes 3, 12, and 17),whereas the remaining 12 offspring inherited the cv Adorra allele(Fig. 3, lane 1 versus lanes 4-11 and 13-16).

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Figure 3. Identification of the $beta$ -amy1 allele in the offspring of the H. spontaneum × Adorra cross. Genomic DNA sequences from the parentscv Adorra (lane 1) and H. spontaneum PI 296897 (lane 2), and fromthe 15 individual lines #1 to #15 (lanes 3-17) were PCR amplifiedfor $beta$ -amy1 intron III-specific sequences. The PCR products weresize fractionated by acrylamide-gel electrophoresis. Lane M, Molecularsize marker.

The total $beta$ -amylase activity in grain from the 15 BC-F₆ lines was also determined and compared with that of the parent lines(Fig. 4). The relative $beta$ -amylase activity of 11 BC-F₆ lines waslower or similar to that of the parent cv Adorra (Fig. 4, bar1 versus bars 3-10, 12, 13, and 15), whereas the relative $beta$ -amylaseactivity of 4 BC-F₆ lines were 27 to 61% higher (Fig. 4, bar 1versus bars 2, 11, 14, and 16), although not to the level of H.spontaneum. Three of these four BC-F₆ lines had inherited theH. spontaneum PI 296897 $beta$ -amy1 allele (Fig. 3, BC-F₆ lines #1,#10, and #15). According to the Mann-Whitney U test (Siegel, 1956)(where U = 2; P < 0.01), the levels of $beta$ -amylase activity measuredin lines carrying the cv Adorra $beta$ -amy1 allele or the H. spontaneumPI 296897 $beta$ -amy1 allele are statistically different. Hence, thedata provide supporting evidence that inheritance of the H. spontaneum $beta$ -amy1 allele is linked to a trait for high $beta$ amylase activityin grain.

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Figure 4. $beta$ -Amylase activity in offspring of the H. spontaneum × Adorra cross. Histogram showing the relative $beta$ -amylase activity ofthe H. spontaneum parent strain (bar 2) and 15 individual lines#1 to #15 (bars 3-17) from the H. spontaneum × Adorra cross normalizedto the $beta$ -amylase activity of the parent cv Adorra (bar 1), calculatedfrom the mean of six independent determinations. The error barsin the histogram represent the SE values. The relative $beta$ -amylaseactivity of cv Adorra of 1.0 is equivalent to a $beta$ -amylase activityof approximately 15 units per 1 mg of protein.

The H. spontaneum PI 296897-Like $beta$ -Amy1 Allele Is Not Found in Modern Barley Cultivars

To study the genetic diversity of the $beta$ -amy1 locus in domesticated barley, we examined several cultivars and lines with differentlevels of $beta$ -amylase activity and known malting characteristics.The allele-specific region of the $beta$ -amy1 intron III, amplifiedby specific PCR primers from genomic DNA, was used to identifythe $beta$ -amy1 allele in relation to the characterized cv Adorra,H. spontaneum PI 296897, and cv Haruna Nijo $beta$ -amy1 alleles (Fig.5). Using this approach the cv Adorra-like 643-bp PCR fragmentwas found in cvs Anisa, Schooner, Steptoe, and Stirling (Fig.5, lanes 1-4 versus lane 5), whereas the H. spontaneum PI 296897-like477-bp PCR fragment (Fig. 5, lane 6) was not seen in modern barley.The cv Haruna Nijo-like 516-bp PCR fragment was found in cvs Alexis,Cork, Kymppi, Morex, Pokko, Triumph, and Vintage (Fig. 5, lanes8-14 versus lane 7).

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Figure 5. Distribution of different $beta$ -amy1 alleles in domesticated barley. The $beta$ -amy1 allele-specific sequence of intron III was PCRamplified from genomic DNA of various barley cultivars. The fragmentswere size fractionated by acrylamide-gel electrophoresis. LaneM, Molecular size marker.

We have not determined the $beta$ -amylase activity of these domesticated barley lines, since our grain samples were harvested fromdifferent locations and years, and their $beta$ -amylase activity wouldthus reflect growth conditions as well as genotype. However, theselected good-malting-quality cultivars (Alexis, Cork, Kymppi,Morex, Pokko, Triumph, and Vintage), known to possess high- $beta$ -amylaseactivity, inherited the cv Haruna Nijo-like $beta$ -amy1 allele (Fig.5), whereas the poorer-malting-quality cultivars (Anisa, Schooner,Steptoe, Stirling, Clipper, Chebec, Bomi, Carlsberg II, GoldenPromise, and Bonus) inherited the cv Adorra-like $beta$ -amy1 allele(Fig. 5 and data not shown). None of the barley cultivars testedinherited the H. spontaneum-like $beta$ -amy1 allele.

Several wild Hordeum spp. collected from different Mediterranean localities were also examined for genetic diversity at the $beta$ -amy1 locus, detected as allele-specific sequence differencesof the $beta$ -amy1 intron III. PCR amplification of the intron IIIregion from genomic DNA samples showed that the wild Hordeum spp.from Cyprus and Corsica and from the areas of Talpiyyot and Meholahad the cv Haruna Nijo-like $beta$ -amy1 allele, whereas the H. spontaneumstrain from the Negev had the cv Adorra-like $beta$ -amy1 allele (datanot shown). Both alleles were found in the H. spontaneum strainfrom Atlit, whereas the H. spontaneum PI 296897-like $beta$ -amy1 allelewas found only in the H. spontaneum strain from the Judean foothills(data not shown).

	DISCUSSION

Top Abstract Introduction Methods Results Discussion References

We are interested in understanding the genetic and molecular mechanisms underlying the variation in $beta$ -amylase activity inthe grain of modern and wild barley. As a part of this work, wehave previously examined 242 accession lines of the wild barleyH. spontaneum and found a wide variation in $beta$ -amylase activities,which were significantly correlated with the annual rainfall patternin their territory of origin (Ahokas and Naskali, 1990b). Thehigh- $beta$ -amylase-activity trait found in H. spontaneum PI 296897has been introduced into the domesticated barley cv Adorra bycrossing (Ahokas and Erkkilä, 1992). Preliminary evidence suggestedthat the backcrossed derivative showing increased enzyme activity(86-H2-64) had inherited a novel $beta$ -amylase allele from H. spontaneumPI 296897.

To gain a closer insight into the $beta$ -amy1 alleles present in the barley gene pool, we performed Southern-blot analysis of the $beta$ -amy1 genes from H. spontaneum PI 296897, cv Adorra, and theirbackcross derivative (86-H2-64), together with the malt barleycv Haruna Nijo. The existence of three distinct $beta$ -amy1 allelespresent in H. spontaneum PI 296897, cv Adorra, and cv Haruna Nijowas indicated, whereas the backcross was shown to have inheritedthe H. spontaneum PI 296897 allele.

We have cloned and sequenced the $beta$ -amy1 alleles from H. spontaneum PI 296897, cv Adorra, and line 86-H2-64 and confirmed thatthe high- $beta$ -amylase trait in the backcross 86-H2-64 is co-inheritedwith the $beta$ -amy1 allele from H. spontaneum PI 296897. The sequencesof the H. spontaneum PI 296897 and cv Adorra $beta$ -amy1 genes andtheir respective transcripts have been compared with each otherand with those of cv Haruna Nijo with the aim of identifying themolecular basis for the different $beta$ -amylase activities found intheir barley grains. The promoter regions of the three alleles,extending approximately 1.3 kb upstream of the ORF, were verysimilar apart from a 25-bp deletion located at the 5 $'$ end of thecv Haruna Nijo promoter fragment. This promoter sequence, encompassingall essential elements required for tissue-specific expressionof the $beta$ -amy1 gene (Kihara et al.. 1997), cannot explain the observeddifferences in $beta$ -amylase activity between cv Adorra and the backcross86-H2-64. Sequence comparisons between the $beta$ -amy1 ORFs of cvsHiproly and Haruna Nijo have previously revealed three amino acidsubstitutions in the deduced sequence (Yoshigi et al., 1994).The deduced amino acid sequence of the H. spontaneum PI 296897ORF shows complete identity to that of cv Haruna Nijo, whereascv Adorra ORF shows two substitutions, Ala-233 $right-arrow$ Val and Ser-347 $right-arrow$ Leu,both of which are found in cv Hiproly. Although Val-233 is a conservativesubstitution, lying in a loop at the protein surface remote fromthe enzyme catalytic site, the nonconservative Leu-347 substitutionmay influence $beta$ -amylase activity, since it involves a polar/nonpolarsubstitution near Glu-345, which lies near the catalytic site(Mikami et al., 1993; Totsuka et al., 1994).

The three $beta$ -amy1 alleles show significant differences, however, in the length and sequence of intron III. The cv Adorra $beta$ -amy1allele has a unique 126-bp insertion, whereas the H. spontaneumPI 296897 $beta$ -amy1 allele has a 39-bp deletion compared with the $beta$ -amy1 intron III of cv Haruna Nijo. To investigate the linkagebetween the high- $beta$ -amylase-activity trait and the allelic natureof intron III of the $beta$ -amy1 gene, we have screened a populationof BC-F₆ lines derived from a single H. spontaneum PI 296897 ×Adorra backcross. After five generations of strong selection fordomesticated morphological features, the remaining populationwas largely composed of lines with $beta$ -amylase activity levels similarto those of cv Adorra. However, three of the four lines exhibitingthe high- $beta$ -amylase-activity trait had the H. spontaneum PI 296897intron III, which, according to the Mann-Whitney U test, establishesgenetic linkage. The high- $beta$ -amylase-activity trait could alsobe attributed to unknown quality trait loci located close to the $beta$ -amy1 locus. Unlinked quality trait loci regulating $beta$ -amylaseactivity may have contributed to the enhanced $beta$ -amylase activityin one line (Hayes et., 1993; Oziel et al., 1996).

The molecular mechanism by which the 126- or 39-bp intron III sequence might influence the qualitative or quantitative expressionof $beta$ -amy1 can only be speculated. Recent reports provide evidencefor transcriptional control elements located within the gene-transcriptionunit, in addition to the promoter elements upstream of the transcriptionalstart site (Bolle et al., 1996; Flieger et al., 1994; Maas etal., 1997). Thus, elements in the 126-bp sequence in intron IIImay bind to a factor(s) that modulates $beta$ -amy1 transcription efficiencyor influences posttranscriptional events such as mRNA maturationand stability. The 126-bp intron III sequence has not previouslybeen found in barley, but shares >85% identity with a part ofthe chloroplastic phosphoglycerate kinase promoter ( $-$ 861 to $-$ 735upstream of the transcriptional start) from wheat (Jones et al.,1995). The 126-bp sequence is composed of a long, inverted repeat,which can be modeled into a stem/loop structure with nucleotides57 to 72 forming an unpaired terminal loop and 14 mismatched nucleotidesin the stem. Further studies will be aimed at providing directevidence for the role of sequence elements within intron III inthe regulation of $beta$ -amy1 at the level of transcription efficiency,mRNA maturation, and/or gene product accumulation.

In the brewing industry DP is an essential parameter of malt quality, since it is a measure of the capacity of the malt todegrade starch into fermentable sugars. Although DP representsthe combined activity of all of the amylolytic enzymes, it isprimarily determined by $beta$ -amylase activity (Santos and Riis, 1996).The PCR analytical technique, developed to distinguish the three $beta$ -amy1 alleles, could provide a valuable breeding tool if it couldbe used to predict DP in barley at the seedling stage. As a firststep in validating this method, a range of poor- and good-malt-qualitybarley lines were screened for intron III structure by PCR, asa means of predicting their $beta$ -amy1 allele identity. Based on theirknown malting quality and published DP measurements (Santos andRiis, 1996), good-quality malting barleys were found to have thecv Haruna Nijo-like $beta$ -amy1 allele, whereas nonmalting barleyshad the cv Adorra-like $beta$ -amy1 allele.

The identification of three $beta$ -amy1 alleles is in agreement with the number of barley $beta$ -amy1 alleles distinguished by IEF.Forster et al. (1991) have identified two alleles at the $beta$ -amy1locus in spring and winter barley genotypes, the $beta$ -Amy1a and $beta$ -Amy1balleles. Analysis of additional cultivars will reveal whether $beta$ -Amy1a and $beta$ -Amy1b alleles correspond to the cv Adorra-like andcv Haruna Nijo-like $beta$ -Amy1 alleles. The third allele was onlyfound in a H. spontaneum strain originating from Judea and inbreeding strains thereof. Chalmers et al. (1992) have analyzedthe different $beta$ -amylase phenotypes present in the H. spontaneumpopulations of Israel. They showed that individual phenotypeswere found in geographical regions where specific environmentalregimes predominate. Thus, the G phenotype is restricted to theNegev Desert and Dead Sea regions, whereas the A phenotype isfound in northern parts of Israel (Chalmers et al., 1992). Wehave shown by the allele-specific PCR approach that H. spontaneumstrains collected from the geographic areas associated with theG phenotype contain the cv Adorra-like $beta$ -amy1 allele, whereasstrains collected from the localities of the A phenotype containthe cv Haruna Nijo-like $beta$ -amy1 allele. We found both $beta$ -amy1 allelesin strains along the Mediterranean coast, where Chalmers et al.(1992) found a heterozygous population, AB.

The H. spontaneum PI 296897-like $beta$ -amy1 allele is not widespread in wild barley, although it is linked to high $beta$ -amylase activityin the grain. Use of this $beta$ -amy1 allele in the modern barley-breedingprogram may contribute to increased levels of grain $beta$ -amylaseactivity in malting barley.

	FOOTNOTES

¹   This research was supported by the Nordisk Forskerutdanningsakademi (grant no. 95.30.075-O).
²   Present address: Plant Breeding Section, Agricultural Research Centre, FIN- 31600 Jokioinen, Finland.
^*   Corresponding author; e-mail verena{at}biobase.dk; fax 45-33-27-47-64.

Received October 20, 1997; accepted March 19, 1998.

ABBREVIATIONS

Abbreviations: DP, diastatic power. ORF, open reading frame.

	ACKNOWLEDGMENTS

We thank Dr. Jacques Rouster, Marja-Riitta Mäkelä, Ella Meiling, Maj-Britt Rask, and Suksawad Vongvisuttikun for genomicDNA samples and technical assistance, and Nina Rasmussen and Ann-SofiSteinholz for help with the figures. We thank Dr. Finn Lok, Dr.Mikael Blom Sørensen, and Dr. David J. Simpson for helpful discussionsand reading the manuscript. We also thank Dr. Yukio Okada (SapporoBrewing, Ltd.) for cv Haruna Nijo grains; Dr. Barbro Jende-Strid(Carlsberg Research Laboratory) for the pro-ant barley line (Anisa);Reino Aikasalo (Boreal Plant Breeding, Jokioinen, Finland) andOuti Manninen and Timo Turpeinen MSc (Agricultural Research Centre)for providing samples of grains and DNA from selected Finnishcultivars, breeding lines, and H. spontaneum strains.

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Allele-Dependent Barley Grain -Amylase Activity1

Copyright Clearance Center: 0032-0889/98/117/0679/07 © 1998 American Society of Plant Physiologists

Allele-Dependent Barley Grain $beta$ -Amylase Activity¹

Copyright Clearance Center: 0032-0889/98/117/0679/07

© 1998 American Society of Plant Physiologists