Abstracts

AGRICULTURAL SCIENCES

Physiological quality and amylase enzyme expression in maize seeds

Qualidade fisiológica e expressão das enzimas amilases em sementes de milho

Gustavo Evangelista Oliveira^I; Renzo Garcia Von Pinho^II; Thaís de Andrade^II; Édila Vilela de Resende Von Pinho^II; Custódio Donizete dos Santos^III; Adriano Delly Veiga^II

^IUniversidade Federal de Lavras/UFLA – Departamento de Biologia/DBI – Cx. P. 3037 – 37200-000 – Lavras – MG – Brasil – gustavo.ufla@gmail.com

^IIUniversidade Federal de Lavras/UFLA – Departamento de Agricultura/DAG – Lavras – MG – Brasil

^IIIUniversidade Federal de Lavras/UFLA – Departamento de Química/DQI – Lavras – MG – Brasil

ABSTRACT

The physiological quality of maize seeds is affected by the genotype. Thus, the study of expression of genes associated with this characteristic is important in the genotype selection process in breeding programs. The aim of this research was to study the expression of amylase enzymes associated with physiological quality of maize seeds with different genotypes and seed sizes. We further sought to assess the expression of these enzymes in dry and soaked seeds The experiment was conducted in the experimental area and the Central Seed Laboratory of the Department of Agriculture of the Universidade Federal de Lavras. Seeds of four maize inbred lines were used, classified in two sizes. The physiological quality of the seeds was evaluated by means of germination, seedling emergence, seedling emergence speed index and accelerated aging test. Expression of the alpha amylase enzyme was evaluated by the electrophoresis technique and expression of the alpha amylase B73, alpha amylase (LOC542522) and beta amylase 5 (amyb5) genes was studied by the qRT-PCR technique in dry and soaked seeds of the inbred lines. There is differentiated expression of amylase enzymes in maize seeds of inbred lines with different levels of physiological quality. higher expression of amylase enzymes is observed in soaked maize seeds. The expression of transcripts is higher in smaller as wellas in soaked maize seeds of inbred lines.

Index terms:Zea Mays, seed quality, qRT-PCR.

RESUMO

A qualidade fisiológica de sementes de milho é influenciada pelo genótipo. Assim, o estudo da expressão de genes associados a essa característica é importante no processo de seleção de genótipos em programas de melhoramento. O objetivo neste trabalho foi estudar a expressão das enzimas amilases associadas à qualidade fisiológica de sementes de milho, de diferentes genótipos e tamanhos de sementes. Objetivou-se ainda avaliar a expressão dessas enzimas em sementes secas e embebidas. O experimento foi conduzido em área experimental e no Laboratório Central de Sementes do Departamento de Agricultura da Universidade Federal de Lavras. Foram utilizadas sementes de quatro linhagens de milho, classificadas em dois tamanhos. A qualidade fisiológica das sementes foi avaliada por meio dos testes de germinação, emergência de plântulas, índice de velocidade de emergência de plântulas e envelhecimento artificial. A expressão da enzima -amilase foi avaliada pela técnica de eletroforese e a expressão dos genes alpha amylase B73, alpha amylase (LOC542522) e beta amylase 5 (amyb5), foi estudada pela técnica de qRT-PCR em sementes secas e embebidas das linhagens. Há expressão diferenciada das enzimas amilases em sementes de linhagens com diferentes níveis de qualidade fisiológica. Maior expressão das enzimas amilases é observada em sementes de milho de menor tamanho e embebidas.

Termos para indexação: Zea Mays, qualidade de sementes, qRT-PCR.

INTRODUCTION

The physiological quality of seeds is affected by the genotype, and thus selection for this characteristic must be considered in genetic breeding programs (GOMES et al., 2000; JOSÉ et al., 2004; HOECHER et al., 2006). In addition, the effect of seed size on the physiological quality of seeds has been observed in some studies (VON PINHO et al., 1995; ANDRADE et al., 1997).

In general, the selection of new cultivars considering the characteristic of seed physiological quality has not been observed in maize breeding programs. Nevertheless, after the value for cultivation and use testing for registering the cultivars, i.e., when the cultivars have already been developed, after several years of selection, one encounters cultivars that are productive but with low physiological quality, which makes placing the new cultivar on the market unviable.

Expression of genes associated with physiological quality may be assessed by means of germination and vigor analyses (COIMBRA et al., 2009; CATÃO et al., 2010) and furthermore by transcriptional analyses of proteins in seeds.

During the maize seed germination process, the embryo produces and secretes natural gibberellins to the endosperm. These hormones induce the development of hydrolytic enzymes in the aleurone layer, such as alpha amylase and beta amylase enzymes, which are responsible for degradation of the reserves that are found in the endosperm. Usually, alpha amylase enzymes are not present in dried seeds, being synthesized "de novo" and secreted by the aleurone layer (KIGEL; GALILI, 1995).

The alpha amylase enzyme is important in starch hydrolysis, being responsible for 90% of amylolytic activity in maize seeds. The alpha amylases constitute a family of endoamylases that catalyze the hydrolysis of -1,4 glycosidic linkages of starch, glycogen and other carbohydrates (FRANCO et al., 2002). This enzyme, together with the beta amylase enzyme is highly related to seed quality. For that reason, gene expression studies of these enzymes, by means of the qRT-PCR (HERNANDEZ et al., 2004; SONG et al., 2011; WANG et al., 2012) and electrophoresis (JOSÉ et al., 2005) techniques are important for knowledge of genetic behavior, thus being able to assist maize genetic breeding programs directed toward seed physiological quality.

Therefore, the aim of this research was to study the expression of amylase enzymes associated with physiological quality of maize seeds with different genotypes and seed sizes. We further sought to assess the expression of these enzymes in dry and soaked seeds.

MATERIAL AND METHODS

The experiments were conducted in the Central Seed Laboratory and experimental area of the Department of Agriculture of the Universidade Federal de Lavras (Federal University of Lavras), municipality of Lavras, MG, Brazil.

Seeds from four inbred lines were discrepant in regard to seed quality according to Gomes et al. (2000), with two being of greater quality (63 and 64) and two of minor quality (43 and 54), table 1.

Initially, a field for multiplication of seeds of the inbred lines was installed by means of self-pollination of the plants. This field consisted of six ten-meter rows for each line, installed at a spacing of 0.8m. Fertilization, management and crop treatments were performed in accordance with that recommended for the crop.

The ears were collected manually when the moisture content of the seeds reached approximately 25%. Husking was performed manually and drying was performed in an ear-corn dryer at a temperature of 35^o C until the seeds reached a moisture content of 13%. After drying and shelling with a manual sheller, the seeds were classified in regard to size in circular sieves and were grouped into seeds retained in the 20/64 and 22/64 pol sieves, designated as large seeds, and those retained in the 18/64 and 16/64 pol sieves, designated as small seeds.

After seed classification, a germination test was performed to verify initial quality of the seeds. Through the results, it could be seen that the seeds from all the inbred lines showed high physiological quality, for the experimental conditions during their production phase were favorable. For selection of discrepant genotypes, just as for physiological quality of the seeds, it was necessary to submit them to accelerated aging. For that reason, the seeds were treated with the fungicide 5,6 - dihydro-2-methyl-1,4-oxathi-ine-3-carboxanilide (200 g/L) and tetramethylthiuram disulfide 200 g/L at a dose of 250 ml for each 100 Kg of seeds. The method used for aging was transparent plastic boxes (11x11x3,5cm), where the seeds were distributed on a screen suspended in the inside of a box containing 40 mL of water, where they remained incubated for 96 hours at a temperature of 41º C (VIEIRA; CARVALHO, 1994). The aged seeds were homogenized and dried in a shaded area at ambient temperature until reaching initial water content of 13%.

Assessment of the physiological quality of the seeds of the four inbred lines was initially performed by means of germination counting in three, five and seven days (BRASIL, 2009), seedling emergence and emergence speed index was performed in plastic box with two parts of soil and one part of sand (EDMOND; DRAPALA, 1958) and accelerated aging test, these tests are according to Gomes et al. (2000).

For analysis of alpha amylase enzyme expression by means of the electrophoresis technique, small and large seeds of the four inbred lines soaked in germitest paper for 70 hours were used. After this period, the embryonic axes were removed and the endosperms were cold ground in liquid nitrogen (ROOD; LARSEN, 1988) and stored in a freezer at -81º C. Another sample of dry seeds was cold ground in liquid nitrogen and stored in a freezer at -81º C up to the time of analysis. Extraction and revelation of the alpha amylase enzyme was performed according to Alfenas (1998).

In addition, analysis of beta amylase and alpha amylase expression was performed by means of the qRT-PCR technique. That way, RNA extraction was carried out from seeds of inbred lines with high and low physiological quality and two sizes, which were crushed in liquid nitrogen and with addition of the reagent Pure Link RNA Plant^® (Invitrogen), according to manufacturer specifications. Integrity of the RNA was verified in 1% agarose gel and viewed after staining with ethydium bromide. RNA quantification was performed in a sprectrophotometer, using wavelengths from 260 and 280 nm.

After nucleic acid extractions, the samples were treated with DNAse Free to avoid any contamination with DNA. Therefore, DNase DNA Free (Ambion) was used and protocol carried out according to manufacturer recommendations. To prove efficiency of decontamination, a conventional PCR reaction was made with all the samples, proving the non-amplification of the DNA. In this reaction, a DNA sample of maize seeds and the primers of the endogenous controls Ubiquitin and Alcohol Dehydrogenase (ADH) were used as positive control. The amplifications were assessed in 1.5% agarose gel stained with ethydium bromide.

After the RNA extraction and purification process, synthesis of cDNA was carried out. For this purpose the High Capacity cDNA Reverse Transcription cDNA^® kit from Applied Biosystems was used, following the protocol recommended by the manufacturer.

For analysis of gene expression by the qRT-PCR technique, the primers used were designed with the assistance of the software Primer Express 3.0 (Applied Biosystems) after a search of the gene sequence at National Center for Biotechnology Information (NATIONAL CENTER FOR BIOTECHNOLOGY INFORMATION-NCBI, 2012), table 2. Ubiquitin and ADH genes (LIVAK; SCMITTGEN, 2001; SCHOLDBERG et al., 2009) were used as endogenous controls.

The equipment ABI PRISM 7500 Real-Time PCR (Applied Biosystems) was used for analysis of quantitative gene expression by qRT-PCR using the detection system SYBR Green and cDNA was obtained from RNA extracted from seeds. Thermal conditions of the reaction were 2 minutes at 50° C, 10 minutes at 95° C, followed by 40 cycles of 15 seconds at 95° C and 1 minute at 60° C, and finalized with 15 seconds at 95° C. The data were collected and stored in the program 7500 software (version 2.0.1). For each reaction, 1.0 μL of cDNA diluted 1:5, 0.2 μL of each primer and 5.0 μL of master mix SYBR green UDG with ROX (Invitrogen) were used for a final volume of 10.0 μL/sample. The negative controls and melting curves were included in all the analyses.

Three technical replications were used for each gene under study, with the results normalized using the Threshold Cycle (CT) obtained by expression of the reference genes ubiquitin and ADH.

CT was determined by the number of cycles in which the fluorescence generated within a reaction crosses the baseline (threshold). The CT comparative method was used. For that purpose, a validation experiment was carried out in advance to prove that the amplification efficiencies of the target genes and references are similar and very near 100% (TYAGI; BRATU; KRAMER, 1998). The standard curves for the genes under study were generated from the following dilutions: 1:5, 1:25, 1:125, 1:625 and 1:3125. This procedure also allowed definition of the best dilution of cDNA used in each reaction, which was 1:5.

The samples of least expression for each gene were used as calibration samples and the method used to measure relative expression was the relative standard curve method, described in the manual of the device (AppliedBiosystems). For quantification of gene expression by the PCR technique in real time, the values obtained corresponding to the mRNA levels of the samples were compared in relation to the values of the control mRNA levels. After obtaining crude data, they were analyzed by means of the 7500 software SDS program (version 2.0.1). To calculate the level of expression of genes of interest, the following were considered: Ct (exponential increase of the PCR product) of the target gene and endogenous control, ΔCt = Ct (sample) – Ct (endogenous control) and the ΔΔCt = ΔCt (sample) - ΔCt (calibrator). Then the level of expression was calculated by the formula: RQ = 2^-ΔΔCt.

For analysis of results of the tests used for assessment of physiological quality, a fully randomized design was used in a 4x2 factorial arrangement, with four inbred lines and two seed sizes, with four replications. Comparison of the means of the treatments for the tests was carried out by the Scott & Knott test at the 5% probability level. Analyses were performed on the statistical program R 2.14.1 (2011).

RESULTS AND DISCUSSION

By the results of analysis of variance of the data obtained in the germination, accelerated aging test, emergence and emergence speed index tests (Table 3), a highly significant (P≤ 0.01) effect was observed for the interaction between the size x inbred line factors and for each isolated factor, with the exception of the emergence speed index, where the size factor was not significant.

The mean values of the data obtained are presented in Tables 4 and 5, together with their groupings by the Scott & Knott test at the 5% probability level.

In the germination test, assessments were performed at three, five and seven days. Lower values of germination at three and five days, regardless of the seed size, were observed in seeds of the inbred lines (43 and 54), defined by Gomes et al. (2000) as being of low quality (Table 4).

In general, in the seeds of inbred line 64, greater mean values of germination were observed in all assessment periods, regardless of size. In small seeds, inferior mean germination values were also observed at seven and five days for inbred lines 54 and 63.

Through the results of the accelerated aging test (Table 5), less vigor was observed in small seeds of inbred lines 43 and 54, and large seeds of inbred line 43. These results are in agreement with those obtained by Gomes et al. (2000), who worked with these same inbred lines and observed that inbred lines 43 and 54 were less vigorous than the others. Less vigor was also observed in small seeds of inbred lines 54 and 64, respectively.

In regard to seedling emergence (Table 5), it was observed that the large seeds of the four inbred lines did not differ among themselves. For the small seeds, lower values were observed in seeds from inbred lines 43 and 63.

The results of the emergence speed index obtained by the formula proposed by Edmond and Drapala (1958) supplies the mean number of days to emergence. It may be observed from the results of Table 5 that for the large seeds, the best indexes were for inbred lines 54 and 63, while for small seeds, the best indexes were observed in seeds of inbred lines 54 and 64.

In general, in the results of tests used for assessment of physiological quality, lower germination and vigor values were observed in seeds of inbred line 43, and better physiological quality in seeds of inbred line 64. It should be noted that depending on the test used, there are some inversions of behavior. According to Gomes et al. (2000), José et al. (2004) and Souza et al. (2008), the physiological quality of maize seeds is controlled by various genes and thus, the conditions during the seed production process may affect the behavior of the inbred line, which requires assessment of quality of seeds produced under different climatic conditions.

The climatic conditions during the seed production process were favorable to the physiological quality of the seeds. For that reason, there was the necessity of submitting the seeds to the accelerating aging before the assessment of physiological quality by the germination and vigor tests. The statistically significant differences observed between nearby germination and vigor values resulting from low values of the coefficient of variation should furthermore be noted (Table 3).

There was a tendency for the large seeds to present mean values greater than the small seeds, just as reported by Carvalho and Nakagawa (2000), who observed greater germination of larger seeds as opposed to the smaller. Nevertheless, there is no consistency of results in the different genotypes, which corroborates the results of Andrade et al. (1997) and Nafziguer (1992). These authors furthermore concluded that the size and format of the maize seeds did not present any significant effect on grain yield.

In figure 1 are presented the isoenzyme patterns of alpha amylase in large and small seeds of maize lines submitted to soaking. Greatest expression of the enzyme was observed in seeds of inbred line 63, and the least expression in those of inbred line 43. The alpha amylase enzyme is important in starch hydrolysis, being responsible for 90% of amylolytic activity in maize seeds (FRANCO et al., 2002). Thus, seeds of genotypes with greater expression of these enzymes have greater ease in making carbohydrates available to the embryo, resulting in greater germination speed and vigor.

In dry seeds, the expression of alpha amylase was not observed by the electrophoresis technique. This is due to the low activity of this enzyme in the dry seeds, with its synthesis by the aleurone layer "de novo" being necessary (KIGEL; GALILI, 1995).

Starch degradation, the main reserve source in most of the seeds of tilled plants, is essential in germination of these seeds (YAMASAKI, 2003). By the results (Figures 1 and 2), it may be observed that the activity of the amylases increases considerably during the soaking process. The same was observed by Sana et al. (2009) working with turnip and wheat seeds.

In relation to seed size, the greatest expression of this enzyme was observed in large seeds of inbred line 54 (Figure 1). In these seeds, greater germination values at 5 and 7 days and greater vigor by the accelerated aging test were observed (Tables 4 and 5).

By the isoenzyme patterns obtained by means of the electrophoresis technique, greater expression of the alpha amylase enzyme in seeds of inbred line 63, regardless of the size, was also observed (Figure 1).

In regard to lower expression of the gene in dry seeds, it is observed that most of the amylase enzymes involved in germination of maize seeds are synthesized "de novo", with the need for soaking. According to Lovegrove and Hooley (2000), Nakajima et al. (2006) and Xie et al. (2007), after soaking, synthesis of gibberellin occurs, which is secreted in the aleurone layer, where it activates alpha amylase synthesis.

In figure 2A, greater expression of the AmyB73 gene is observed in soaked seeds of inbred line 64. Expression of this gene was not observed in dry seeds in any of the inbred lines, and in this situation there is "de novo" synthesis of the enzyme after soaking of the seeds (KIGEL; GALILI, 1995). This behavior was also observed for the alpha amylase gene (LOC542522), with greater expression in soaked seeds of inbred line 63 (Figure 2B).

It may be inferred that the AmyB73 and alpha amylase (LOC542522) genes are associated with the physiological quality of seeds of the inbred lines studied. For lines 64 and 63 classified as having seeds of greater physiological quality, the greatest values of expression of the AmyB73 and alpha amylase (LOC542522) genes were observed, respectively. By means of germination and vigor tests, lower physiological quality was observed in seeds of inbred line 43. For these two genes in this inbred line, the lowest expression was observed. It should be noted that in this inbred line there was expression of the alpha amylase (LOC542522) gene only in the large and soaked seeds.

In relation to the AmyBeta5 gene (Figure 2C), its expression was observed only in the soaked seeds. Moreover, greater expression was observed in small soaked seeds. The beta amylase enzyme is synthesized during seed development and its release and activation occurs during germination, being accompanied by the accumulation of its isoforms (SOPANEN; LAURIÈRE, 1989). The gene in reference is related to synthesis of beta amylase in the literature. Nevertheless, its expression was not observed in dry seeds.

Comparing the results of the expression observed by the qRT-PCR and electrophoresis techniques, specific isoforms which may be associated with the genes under study are verified in the alpha amylase zymogram (Figure 1). It is inferred that the AmyB73 gene (Figure 2A) is associated with isoform 1 of alpha amylase and the alpha amylase (LOC542522) gene (Figure 2B) is associated with isoform 2 of alpha amylase.

Furthermore, in relation to the zymogram presented in figure 1, greater activity of the alpha amylase enzyme is observed for inbred line 63, and upon comparing these results with the expression assessed by the qRT-PCR technique, greater expression of the alpha amylase (LOC542522) and AmyBeta5 genes is observed (Figure 2).

Thus, upon assessing amylase enzyme expression by means of the electrophoresis and qRT-PCR techniques and by the results of tests used for assessment of physiological quality, it is observed that inbred line 43 presents lower physiological quality, which could compromise its use in hybrid composition, principally as a female parent. Thus, by means of these analyses, there was significant expression of genes associated with amylase enzymes and with physiological quality of the seeds.

Analysis of the alpha amylase enzyme expression profile by means of the electrophoresis technique may be used to assist selection of genotypes in breeding programs. That way, it is possible to eliminate genotypes with minor seed quality in the initial phases of the program.

It is important to emphasize that various genes in addition to the amylases may be involved in control of the seed physiological quality trait. For example, genes directly related to plant respiration may be cited. Therefore, it is suggested that new studies be carried out seeking to involve a greater number of multigene families and genes.

CONCLUSIONS

There is differentiated expression of amylase enzymes in maize seeds of inbred lines with different levels of physiological quality.

Higher expression of amylase enzymes is observed in soaked maize seeds.

The expression of transcripts is higher in smaller as well as in soaked maize seeds of inbred lines.

ACKNOWLEDGEMENTS

To the National Council of Scientific and Technological Development (Conselho Nacional de Desenvolvimento Científico e Tecnológico - CNPq), CAPES and the Research Support Foundation of the State of Minas Gerais (Fundação de Amparo à Pesquisa do Estado de Minas Gerais - FAPEMIG) for financial support.

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(Received in october 27, 2012 and approved in december 12, 2012)

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