Temperature-Induced Extended Helix/Random Coil Transitions in a Group 1 Late Embryogenesis-Abundant Protein from Soybean

doi:10.1104/pp.010521

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Temperature-Induced Extended Helix/Random Coil Transitions in a Group 1 Late Embryogenesis-Abundant Protein from Soybean¹

Jose L. Soulages, Kangmin Kim,² Christina Walters, and John C. Cushman^*

Department of Biochemistry and Molecular Biology, 355 Noble Research Center, Oklahoma State University, Stillwater, Oklahoma 74078-0454 (J.L.S.); Department of Biochemistry, 311B Fleischmann Agriculture, University of Nevada, Reno, Nevada 89557-0014 (K.K., J.C.C.); and National Seed Storage Laboratory, United States Department of Agriculture-Agricultural Research Service, Fort Collins, Colorado 80523 (C.W.)

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
RESULTS
DISCUSSION
MATERIALS AND METHODS
LITERATURE CITED

Group 1 late embryogenesis-abundant (LEA) proteins are a subset of hydrophilins that are postulated to play important rolesin protecting plant macromolecules from damage during freezing,desiccation, or osmotic stress. To better understand the putativefunctional roles of group 1 LEA proteins, we analyzed the structureof a group 1 LEA protein from soybean (Glycine max). Differentialscanning calorimetry of the purified, recombinant protein demonstratedthat the protein assumed a largely unstructured state in solution.In the presence of trifluoroethanol (50% [w/v]), the protein acquireda 30% $alpha$ -helical content, indicating that the polypeptide is highlyrestricted to adopt $alpha$ -helical structures. In the presence of sodiumdodecyl sulfate (1% [w/v]), 8% of the polypeptide chain adoptedan $alpha$ -helical structure. However, incubation with phospholipidsshowed no effect on the protein structure. Ultraviolet absorptionand circular dichroism spectroscopy revealed that the proteinexisted in equilibrium between two conformational states. Ultravioletabsorption spectroscopy studies also showed that the protein becamemore hydrated upon heating. Furthermore, circular dichroism spectralmeasurements indicated that a minimum of 14% of amino acid residuesexisted in a solvent-exposed, left-handed extended helical orpoly (L-proline)-type (PII) conformation at 20°C with the remainderof the protein being unstructured. The content of PII-like structureincreased as temperature was lowered. We hypothesize that by favoringthe adoption of PII structure, instead of the formation of $alpha$ -helicalor $beta$ -sheet structures, group 1 LEA proteins retain a high contentof surface area available for interaction with the solvent. Thisfeature could constitute the basis of a potential role of LEAproteins in preventing freezing, desiccation, or osmotic stressdamage.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION RESULTS DISCUSSION MATERIALS AND METHODS LITERATURE CITED

Late embryogenesis-abundant (LEA) proteins accumulate to high concentrations in plant embryos during the latter stages ofseed development before desiccation (Baker et al., 1988; Dureet al., 1989; Hughes and Galau, 1989). LEA proteins also accumulatein vegetative tissues exposed to exogenous abscisic acid, as wellas dehydration, osmotic, and low-temperature stress (Chandlerand Robertson, 1994; Ingram and Bartels, 1996; Bray, 1997; Close,1996, 1997; Thomashow, 1998; Nylander et al., 2001). More thanseven different groups of LEA proteins have been described andcategorized by virtue of similarities in their deduced amino acidsequences (Baker et al., 1988; Dure et al., 1989). The majorityof LEA proteins are highly hydrophilic and display a preponderance(e.g. Ala, Gly, Glu, and Thr) or lack (e.g. Trp and Cys) of certainamino acid residues (Dure, 1993a, 1993b, 1997). Thus, LEA proteinsare part of a larger, evolutionarily conserved group of hydrophilicproteins termed "hydrophilins" involved in various adaptive responsesto hyperosmotic conditions (Garay-Arroyo et al., 2000).

Various functions have been proposed for different groups of LEA proteins ranging from water binding to minimize water lossand protein and membrane stabilization or protection to ion sequestrationand scavenging (Dure, 1993a, 1993b; Close, 1997; Danyluk et al.,1998). LEA proteins also display diverse subcellular and tissue-specificlocalization patterns, suggesting that different groups or groupmembers fulfill specific functional roles (Close, 1997; Nylanderet al., 2001). LEA protein expression generally correlates wellwith desiccation tolerance in young seedlings (Bartels et al.,1988; Reid and Walker-Simmons, 1993; Whisitt et al., 1997) aswell as salt tolerance (Moons et al., 1995) and freezing tolerance(Houde et al., 1995; Van Zee et al., 1995; Close, 1997; Danyluket al., 1998). Furthermore, ectopic expression of a barley (Hordeumvulgare) group 3 LEA protein, HVA1, in transgenic rice (Oryzasativa) improved tolerance to salinity and drought stress (Xuet al., 1996). When expressed in yeast (Saccharomyces cerevisiae)cells, HVA1 improved growth rates under ionic (NaCl and KCl) stressas well as improving cell freezing tolerance (Zhang et al., 2000).Overexpression of a tomato (Lycopersicon esculentum) group 2 (le4)and group 4 protein (le-25) conferred improved yeast cell growthrates at high NaCl and KCl concentrations, respectively, withboth proteins improving freezing tolerance (Imai et al., 1996;Zhang et al., 2000). Similarly, overexpression of a group 1 LEAprotein from wheat (Triticum aestivum; Em) in yeast cells resultedin improved growth under high NaCl, KCl, and sorbitol conditions(Swire-Clark and Marcotte, 1999). These observations suggest thatdifferent LEA proteins may play distinct but related roles inameliorating different stress effects. However, the exact in plantafunction of these different groups of LEA proteins remainunknown.

Group 1 LEA proteins are distinguished from other groups of LEA proteins by being very hydrophilic and highly conserved alongthe entire length of the protein (Dure, 1993, 1997). Group 1 LEAproteins are further characterized by having an internal 20-aminoacid signature motif repeated up to four times depending on thespecies (Esperlund et al., 1992) and a high proportion of Gly,Glu, and Gln residues. These signature repeats are evident inthe Bacillus subtilis GsiB stress protein (Stacy and Aalen, 1998),which is induced by Glc or phosphate starvation, oxygen limitation,heat, oxidation, and salinity (Völker et al., 1994). Such remarkableconservation suggests an important role in stressadaptation.

The predicted hydrophilic and high degree of random coil structure of group 1 LEA proteins have led some researchers to proposethese proteins may serve as water-binding proteins that can minimizewater loss (McCubbin et al., 1985; Roberts et al., 1993), actas hydration buffers to regulate water status (Dure, 1993a; Walterset al., 1997), or interact with the surface of macromoleculesas a water matrix or replacement to oppose protein denaturationin dehydrating tissues (McCubbin et al., 1985; Cuming, 1999).However, few biochemical analyses using purified group 1 LEA proteinshave been reported. Circular dichroism (CD) spectroscopy and hydrodynamicmodeling suggested that the wheat group 1 LEA protein, Em, contains70% random coil or non-regular, flexible secondary structure (McCubbinet al., 1985). NMR spectroscopy of a recombinant carrot (Daucuscarota) group 1 protein, EMB-1, expressed in Escherichia colirevealed no defined secondary or tertiary structure of the proteinin solution (Eom et al., 1996). However, understanding the detailedmechanisms by which group 1 LEA proteins may confer protectionagainst osmotic stress will require more specific informationabout the biochemical and biophysical properties of these proteins.Here, we examined the structural properties of a highly purified,recombinant group 1 LEA protein from soybean (Glycine max; rGmD-19).UV absorption and CD spectroscopy studies performed under a rangeof temperatures and pH revealed that the protein is largely unstructuredwith 6% to 14% of the protein occupying a left-handed extendedhelical or poly (L-Pro)-type (PII) conformation. Furthermore,the protein was found to exist in equilibrium between two conformationalstates with a low degree of transitionalcooperativity.

	RESULTS

TOP ABSTRACT INTRODUCTION RESULTS DISCUSSION MATERIALS AND METHODS LITERATURE CITED

Overexpression and Purification of rGmD-19

To study the structural and physicochemical characteristics of group 1 LEA from soybean in detail, large (milligrams) quantitiesof the recombinant soybean D-19 (rGmD-19) protein were producedand purified from E. coli. Affinity tag sequences were removedfrom the pET30a expression vector to express the native protein.From total cell lysates of E. coli BL21 (DE3) plysS cells, weobserved the induction of the putative GmD-19 gene product withan apparent molecular mass of 11.4 kD (Fig. 1A).

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Figure 1. Expression and purification of group 1 LEA protein from E. coli. A, rGmD-19 accumulation at different times after isopropylthio- $beta$ -galactoside (IPTG) induction. Protein overexpression was induced with 0.1 mM IPTG when the optical density (OD)₆₀₀ was 0.8. Cells were collected at various time points and soluble proteins were extracted. Con, No IPTG; 1, induction point, 120 min; 2, 135 min; 3, 150 min; 4, 180 min; 5, 210 min; 6, 240 min; 7, 270 min; 8, 300 min; 9, 360 min. Approximately 10 µg of protein was loaded in each lane. B, Composite purification steps of rGmD-19 treated with boiling. Approximate amount of protein loaded in each lane is indicated in parentheses. TL, Total lysate (10 µg); BT, boiling treated (5 µg); IF, isoelectric focusing (IEF; 2 µg); HQ, high Q (1.5 µg). C, Composite purification steps of rGmD-19 without boiling. TL, Total lysate (10 µg); SO, 60% (w/v) (NH₄)₂SO₄ salting out (10 µg); IF, IEF (2 µg); HQ, high Q (2 µg); HS, high S (1.5 µg). Line designates rGmD-19. The relative mass of prestained or stainable molecular mass standards are designated in kilodaltons (kD).

Initial purification took advantage of the unique property of rGmD-19 solubility after exposure to boiling conditions. Subsequentpurification steps included preparative IEF and anion-exchangechromatography, which were needed to achieve a high degree ofpurification (Fig. 1B). To determine whether rGmD-19 structurewas altered by heat denaturation, rGmD-19 protein was also purifiedwithout boiling. Precipitation at 60% (w/v) (NH₄)₂SO₄ was substitutedfor heat and used as the initial purification step. PreparativeIEF and anion-exchange column chromatography steps followed; however,it was necessary to include an additional cation exchange columnchromatography step to attain homogeneity (Fig. 1C). Both rGmD-19spurified using heat and (NH₄)₂SO₄ showed identical electrophoreticmobility after analysis by native or denaturing SDS-PAGE (datanot shown). The identity of the proteins purified by either purificationstrategy was confirmed by matrix-assisted laser-desorption ionizationtime of flight mass spectrometry (MS). The molecular mass of rGmD-19was 11.359 kD, which is identical to the predicted molecular mass11.359 kD (without N-terminal f-Met). Both noninduced E. colicells and cells induced for rGmD-19 overexpression showed similargrowth rates, suggesting that rGmD-19 protein accumulation wasnot harmful to cell viability (data notshown).

Thermal Stability of rGmD-19

Differential scanning colorimetry (DSC) was used to investigate a potential cooperative structural transition of rGmD-19.The DSC scans in Figure 2A show a typical denaturation patternof a heat-labile protein (e.g. BSA). BSA undergoes thermal denaturationaround 80°C. In contrast, DSC scans of rGmD-19, purified withor without boiling, show no detectable high-temperature peak (Fig.2B). This result suggests that the protein failed to undergo anydetectable irreversible denaturation. Similar results have beenreported for a group 1 LEA protein isolated from pea (Pisum sativum)embryonic axes (Russouw et al., 1997). These DSC results are alsoconsistent with previous studies indicating a low proportion ora lack of distinct tertiary structure in group 1 LEA proteins(McCubbin et al., 1985; Eom et al., 1996). Even though heatingmay alter the structure of rGmD-19 on a molecular scale, suchchanges may be of low cooperativity and thus not detectable byDSC. Therefore, spectroscopic methods, more sensitive at detectingmolecular scale changes in structure, were tested.

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Figure 2. Heating thermograms of bovine serum albumin (BSA) and rGmD-19 using DSC. DSC heat scans of BSA (A) or rGmD-19 (B) with and without boiling treatment (BT) were performed at 10°C min¹ from 0°C to 100°C. Plots of each scans were offset slightly for clarity. HTP, High temperature peak.

UV Absorption Spectroscopy

rGmD-19 contains only two aromatic residues, one Tyr at position 57 and one Phe at position 89. Therefore, the near-UV absorptionspectrum should be dominated by the absorption characteristicsof the Tyr residue. The UV absorption spectrum of rGmD-19 showedtwo absorption maxima located at 228 and 275 nm (Fig. 3). Themaximum at 275 nm is characteristic of the absorption by Tyr andconfirms the absence of Trp. The maximum at 228 nm is dominatedby the absorption of Tyr, but probably also has a contributionfrom the absorption of Phe and His residues (Demchenko, 1986).

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Figure 3. UV absorption spectrum of rGmD-19 (77 µM) in 50 mM phosphate buffer, pH = 7, 24°C. The inset shows the expanded near-UV region of the spectrum.

Secondary Structure of rGmD-19

The secondary structure of rGmD-19 in solution was estimated from the far-UV CD spectrum at different temperatures and pHs.The CD spectra of rGmD-19 at pH 5, 8, and 9 remained unchanged(data not shown), indicating that in this pH range the structureof the protein was not modified. A simple inspection of the CDspectra of rGmD-19 shows a strong negative band at 200 nm, whichis generally found in highly unfolded proteins (Woody, 1992).The structural composition of the protein was estimated by themethod of Sreerama et al. (1999), using a reference data set of37 proteins that included the CD spectra of five unfolded proteins.The results obtained at 20°C (Table I) indicated that this proteinhas a very low content of the typical secondary structural elementsof $alpha$ -helices or $beta$ -strands and a high content of "unordered" structure.

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Table I. Secondary structure fractions of rGmD-19
The fractions were determined by the method of Sreerama et al. (1999)

. Data were acquired at pH = 7 and 20°C.

Temperature-Induced Structural Changes Monitored by UV Absorption

Temperature-induced changes in the hydration of the Tyr residue of rGmD-19 were studied by second derivative UV absorptionspectroscopy. This method is a reliable, quantitative, and sensitivetool to study the hydration of aromatic residues (Ragone et al.,1984; Demchenko, 1986; Soulages and Bendavid, 1998). Using Tyrfluorescence spectroscopy, Russouw et al. (1997) reported no differencein the Tyr environment of a group 1 LEA protein from pea beforeand after heat treatment (80°C). In contrast to this earlier work,Figure 4A shows the spectral changes that occur when the temperaturewas increased from 10°C to 80°C. In the spectral region displayed,the temperature-induced changes observed in the second derivativespectrum of rGmD-19 reflect the changes in the hydration of theTyr residue. Even though the Tyr residue was highly hydrated at10°C, the spectral changes observed indicate that the proteinbecomes more hydrated as the temperature is increased. These changessuggest that heating promotes a structural transition involvingan unfolding process. In addition to the changes in the intensityof the second derivative spectra, another important feature observedin this study is the presence of several isobestic points (Fig.4A). The presence of an isobestic point indicates a transformationinvolving two components. The fact that these isobestic pointsremain unchanged in the entire range of temperatures studied suggeststhat, in the 12°C to 80°C temperature range, there is an equilibriumbetween two conformational states. Because second derivative spectraobey Beer's law, as well as zero order spectra (Demchenko, 1986),we can use the difference between the second derivative valuesat any two given wavelengths as a measure of the relative changein the population of the conformational states. We have done thisusing the values of the derivative at 279 and 283 nm. Figure 4Bshows that between 12°C and 80°C there is a continuous changein $Delta$ (279-283) [ $delta$ ² $epsilon$ / $delta$ $lambda$ ²]. Consistent with the DSC results, the slope of the plot suggeststhat the cooperativity of this conformational transition is quitelow.

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Figure 4. Effect of temperature on the second derivative spectrum of rGmD-19. A, The spectra shown, reading downward at 283 nm, represent increasing temperatures from 14°C to 78°C. The temperatures are indicated in the figure. B, The temperature-induced changes are represented using the difference between the derivative values at 279 and 283 nm: $Delta$ (279-283) [ $delta$ ² $epsilon$ / $delta$ $lambda$ ²].

Effect of SDS Micelles, Phospholipid Liposomes, and Trifluoroethanol (TFE) on the Secondary Structure of rGmD-19

Even though rGmD-19 exhibited a very low degree of structural organization in aqueous medium, we studied its tendency to adopthelical structure by determining the CD spectrum in a solutioncontaining 50% (v/v) of TFE, a helix-promoting solvent. In thepresence of 50% (v/v) TFE, rGmD-19 acquired a significant degreeof $alpha$ -helical structure (Fig. 5). The difference spectrum has thetypical features of an $alpha$ -helical polypeptide (Fig. 5, inset).Using the difference spectrum it is estimated that, at 50% (v/v)TFE, the $alpha$ -helical content of the protein is approximately 30%.This estimate indicated that the primary structure of the proteinimposes significant restrictions to the adoption of $alpha$ -helicalstructures. Using a similar approach, the Em protein from wheatwas previously shown to increase in $alpha$ -helical content from 13%to 29% in the presence of 45% (v/v) TFE (McCubbin et al., 1985).

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Figure 5. Effect of SDS and TFE on the secondary structure of rGmD-19. The CD spectra of rGmD-19 were obtained in 5 mM sodium phosphate buffer, pH 6.5, at room temperature. The samples of rGmD-19 containing SDS or TFE were prepared 1 h before the acquisition of the spectra. The inset shows the difference spectra that were obtained after subtracting the spectrum of rGmD-19 in buffer from the spectra obtained with either SDS or TFE.

Ismail et al. (1999) have observed that a group 2 LEA (dehydrin) protein from cowpea (Vigna unguiculata) acquired $alpha$ -helicalstructure in the presence of SDS, suggesting that this proteinmay contain $alpha$ -helical structures in a lipid-bound state in vivo.To determine if the structural properties of rGmD-19 might beinfluenced by lipid interactions, we tested the effect of SDSand unilamellar liposomes of dimyristoyl phosphatidylcholine onrGmD-19 structure. The CD spectra of rGmD-19 in the presence ofSDS (Fig. 5), and the difference spectrum (spectrum in the presenceof SDS minus spectrum in the absence of SDS), indicated that theprotein interacts with SDS micelles and gains some $alpha$ -helical structure.In the presence of detergent, the protein contains 8% of $alpha$ -helicalstructure. Because SDS micelles have a very high charge density(negative), their interaction with the protein may not be physiologicallyrelevant. To investigate whether the protein could interact withother lipid surfaces, we also incubated rGmD-19 with unilamellarliposomes of dimyristoyl phosphatidylcholine at a 20:1 lipid:proteinmolar ratio. This incubation produced no changes in the CD spectrumof rGmD-19 (data not shown), suggesting that the protein is unableto interact with zwitterionic phospholipid membranes. This resultis in agreement with previous studies showing the lack of a specificphospholipid-protein interaction of other cold-induced proteins(Uemura et al., 1996; Webb et al., 1996). Although these resultscannot discount the possibility that this group 1 LEA proteinmay interact with and be influenced by interaction with membranelipids in vivo, we suggest that such interactions are unlikelygiven the extremely hydrophilic nature of thisprotein.

Temperature-Induced Structural Changes Monitored by CD

Earlier investigations of a pea group 1 LEA protein using CD spectroscopy showed that heat treatment had no effect on theCD spectrum of the protein (Russouw et al., 1997). To more thoroughlyinvestigate possible temperature- induced structural changes inrGmD-19, we obtained CD spectra at several temperatures (Fig.6A). Contrary to the effect of pH, raising the temperature promotedsignificant changes in the CD spectrum of rGmD-19. Deconvolutionof the spectra obtained at different temperatures by the methodof Sreerama et al. (1999) renders no significant changes in thefractions of different secondary structural elements. Despitethis, and although there are no changes in the shape of the spectrum,increasing the temperature produces a gradual and significantincrease in the negative band centered between 210 and 230 nmas well as a concomitant decrease in the intensity of the negativeband centered at 200 nm. Besides the changes in these two negativebands, it is also evident that at approximately 208 nm and $-$ 7,900degree cm² dmol¹, there is an isodichroic point. This point is maintained in thetemperature range studied, 10°C to 80°C, suggesting the presenceof an equilibrium between two conformational states (Fig. 6B).This observation is consistent with the isobestic points observedby UV absorption and provides further support to the existenceof a two-state equilibrium.

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Figure 6. Effect of increasing temperature on secondary structure of rGmD-19. A, CD Spectrum of rGmD-19. The CD spectrum was acquired in a 7.7 µM protein solution in 50 mM buffer Na-phosphate. The spectra shown, reading downward at 220 nm, represent increasing temperatures: 10°C, 20°C, 30°C, 35°C, 40°C, 50°C, 55°C, 60°C, 65°C, 70°C, 75°C, and 80°C. The inset shows the convergence of the ellipticities at 208 nm. B, The temperature-induced changes in the CD spectrum are represented using the ellipticity values obtained at 208 and 215 nm. Symbols are indicated in the figure.

The decrease in intensity of the 200-nm band, and the increase in intensity of the band near 220 nm (Figs. 6A and B), whichare characteristic of an increase in $alpha$ -helical content, led usto consider the possibility that increased temperature-inducedfolding of the protein rather than unfolding. However, the factthat the increase in temperature was accompanied by an increasein the hydration of the protein, as inferred from the UV absorptionstudy, indicated that this possibility was not likely. In fact,the changes observed by UV absorption spectroscopy are indicativeof an unfolding process. As indicated below these changes weredue, in fact, to an unfoldingprocess.

Evidence of an Extended Helix Conformation

The difference spectrum ( $Delta$ 10°C-75°C) of rGmD-19 is shown in Figure 7. This difference spectrum is characterized by an intensenegative CD band centered at 200 nm, and a positive CD band above200 nm. The positive band indicates that the contribution of $alpha$ -helicalstructures to the CD spectrum is very low. Otherwise, we shouldexpect a decrease in $alpha$ -helical content as the temperature increases,and a negative CD band above 200 nm in the difference spectrum.It is interesting that these two features observed in the differencespectrum are present in the CD spectra of peptides rich in poly(Pro)II-like (PII) structures (Park et al., 1997). This similaritysuggested that the spectral changes observed in rGmD-19 couldbe because of a temperature-induced extended helix/random coiltransition. The difference spectrum shows a maximum at 215 nm,which is coincident with the maximum observed in peptides adoptingPII-like conformations. Additional support for this possibilityarises from the coordinates of the isodichroic point observedin Figure 6A (208 nm and $-$ 7, 900 deg cm² dmol¹). These coordinates are coincident with the coordinates observedin model peptides that undergo PII/random coil transitions (Woody,1992).

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Figure 7. CD difference spectrum. The CD component that disappears upon heating is illustrated in the graph by the CD difference spectrum between (CD at 10°C $-$ CD at 75°C).

Park et al. (1997) have investigated a series of host/guest peptides and suggested limiting values of ellipticity for thePII and the unordered structures of +9,580 and $-$ 5,560 deg cm² dmol¹ at 222 nm. Using these suggested values, we can estimate thefractions of unfolded and PII conformations in rGmD-19 at differenttemperatures. To perform this calculation, we also assumed thatthe $alpha$ -helical content of the protein was nearly zero at high andlow temperatures. This assumption appears to be well supportedby the maintenance of the isodichroic point along the entire temperaturerange studied. If this transition would involve three states,unordered, $alpha$ -helical, and PII, one should not expect the maintenanceof the isodichroic point. Using these limiting values, and theellipticity of rGmD-19 at pH 7.0 and 10°C, we inferred that rGmD-19contains a minimum of 14% of its residues in an extended-helixconformation. This fraction would be reduced to 6% at 80°C. Thisestimation represents a minimum estimate because the presenceof a small amount $alpha$ -helical structure would decrease significantlythe estimation of the PII-likestructure.

	DISCUSSION

TOP ABSTRACT INTRODUCTION RESULTS DISCUSSION MATERIALS AND METHODS LITERATURE CITED

Previous in vivo functional studies of a group 1 LEA protein from wheat have shown that this protein can ameliorate the detrimentaleffects of ionic or osmotic stress in yeast cells (Swire-Clarkand Marcotte, 1999). Despite these observations, the mechanismsby which this protein acts to afford such protection remain largelyunknown. Predicted structural features of group 1 LEA proteinsand their highly hydrophilic nature have led researchers to suggestthat this group of highly conserved proteins protect cells ortissues from damage by maintaining or replacing water at the interactioninterface with other macromolecules (McCubbin et al., 1985; Dureet al., 1989; Cuming, 1999). However, detailed in vitro biochemical,physicochemical, and structural analyses are needed to gain aclearer picture of how group 1 LEA proteins function. Toward thisend, we have purified large amounts of soybean group 1 LEA proteinfrom E. coli to initiate detailed structural analyses. We firstused DSC scans to determine if rGmD-19 showed a cooperative unfoldingtransition characterized by a heat absorption band. In contrastto BSA, rGmD-19 showed no heat absorption peaks in DSC scans from10°C to 100°C. This result was independent of whether the proteinwas purified by heat denaturation or (NH₄)₂SO₄ precipitation (Fig.2B). These DSC results of rGmD-19 are entirely consistent withthe secondary structure analysis of CD data, which showed thatthe protein assumes a largely unordered structure in solution.This observation is also consistent with previous hydrodynamicand CD or NMR spectroscopy studies, which reported that group1 LEA proteins possess little or no apparent defined secondarystructures (McCubbin et al., 1985; Eom et al., 1996). One-dimensionalNMR analysis of a group 1 protein (EMB-1) from carrot indicatedthat its polypeptide backbone was extremely flexible on a sub-nanosecondtime scale (Eom et al., 1996). Attempts to induce structure inthe EMB-1 protein by approximating dehydration conditions withTFE and ethanol failed to demonstrate any identifiablestructure.

The major finding of this study is that we demonstrated that rGmD-19 actually undergoes a temperature-induced structural transition.Moreover, we show that low temperatures favor the adoption ofa PII structure. PII helices are secondary structural elementsimportant for many structural proteins, in unfolded proteins,and in protein-protein interaction domains (Creamer, 1998; Stapleyand Creamer, 1999). Most PII helices are only five to 12 aminoacids in length, and their formation is favored by Pro residues;however, Gln and positively charges amino acids, which compose30% of GmD-19 amino acids, also favor their formation. Our studyalso shows that the temperature-induced spectroscopic changesobserved in rGmD-19 are because of the equilibrium between anextended-helix conformation, PII, and a random coil or unorderedconformation. Similarly, Lisse et al. (1996) reported that a dehydrin-likeLEA protein (Dsp16) underwent temperature- and denaturant-dependentorder-disorder structural transitions. However, PII structureswere not identified in this report. Furthermore, one-dimensionalNMR studies suggested the presence of interactions within thepolypeptide chain that might stabilize or slow the rapid equilibriumbetween conformational states, but no PII structures were elucidated(Lisse et al., 1996). Our preliminary results suggest that a relatedgroup 2 LEA protein from soybean (DHN1) undergoes structural transitionssimilar to both rGmD-19 and Dsp16 (J. Soulages, unpublished data).Thus, the adoption of PII structures might be a common propertyof group 1 and 2 LEA proteins. To our knowledge, experimentalevidence supporting the presence of PII structures in any LEAproteins has not been previouslyreported.

Large regions of random coil conformation are considered to promote the efficient interaction of group 1 LEA proteins withwater and aid in their ability to prevent cellular water loss(McCubbin et al., 1985; Eom et al., 1996; Cuming, 1999). The highdegree of random coil formation in rGmD-19 structure suggestsit can fulfill such a role. In addition, PII helices are highlysolvent exposed and are expected to contribute to solvent interactions.Because of the distribution of highly polar amino acid residues,rGmD-19 may also be able to serve as a partial replacement forwater in desiccated cell (Crowe et al., 1992; Cuming, 1999). Eventhough the biochemical roles of PII structures have not been firmlyestablished, the fact that decreasing the temperature inducesan increase in the structural organization of the protein withoutcompromising the interaction of the protein with the solvent constitutesan indication about a potential role of the PII structure andof GmD-19 in protection against freezing, desiccation, or osmoticstress damage. Thus, although the content of PII structure increasessignificantly as the temperature decreases, there is no increasein the apparent content of $alpha$ -helical or $beta$ -structures, which woulddecrease the number of potential interactions between the solventand the protein backbone. Compared with a random coil structure,the $alpha$ -helical or $beta$ -sheet structures represent a dramatic decreasein the number of H-bond interactions between the solvent and thepolypeptide backbone as well as a decrease in the exposed surfacearea of hydrophobic and hydrophilic residues. However, the extendedhelical conformation of the PII structure retains a high degreeof exposed surface area. It has been estimated that residues withinPII helices expose between 50% and 60% more surface area thando average residues (Adzhubei and Sternberg, 1993).

PII structures are also found in certain glycosylated polar fish antifreeze proteins (Bush et al., 1984; Lane et al., 1998,2000). Antifreeze glycoproteins (AFGP) are responsible for non-colligativefreezing point depression, inhibition of ice nucleation and crystalgrowth in aqueous solutions, and differentially effect membranestability during freezing (Yeh and Feeney, 1996; Davies and Sykes,1997; Tomczak et al., 2001). AFGP8 has a slight cryoprotectiveeffect against freezing-induced membrane leakage. Similar to group1 LEA proteins, AFGP8 has no long-range ordered structure andhas significant flexibility (Lane et al., 1998, 2000). One possiblemechanism for AFGP action is to promote cooperative hydrogen bondingover its length sufficient for disruption of ice crystal growth(Yeh and Feeney, 1996). Unlike fish AFGPs, our mass spectrometrymeasurements of rGmD-19 demonstrated that it lacks glycosylation.Furthermore, computer-assisted motif searches for posttranslationalmodification motifs confirmed that rGmD-19 lacks consensus glycosylationmotifs. This is important because the antifreeze property of theglycoproteins from arctic fish is most often attributed to thewater-carbohydrate interactions via hydrogen bonding, rather thanto water-peptide interactions. However, despite the absence ofglycosylation, we suggest that in a hydrophilic protein that isrich in PII structure at low temperatures, the peptide backboneand side chains could act as an efficient protectant against dehydration,osmotic, and/or freezing damage. Deeper insights into the mechanismof action of group 1 LEA proteins should come from two-dimensionalor multidimensional NMR studies leading to a solution structure.Such information would be useful in the development of modelingalgorithms for predicting PII structures (Creamer, 1998; Siermalaet al., 2000). This information could also be used to developa molecular model for the interaction between the amino acid sidechains and backbone with water in thefuture.

Many unordered proteins or domains can adopt a well-defined structure upon binding to target molecules. Recent observationsby Ismail et al. (1999) showed that a group 2 LEA (dehydrin) proteinfrom cowpea can adopt increased $alpha$ -helical content in the presenceof SDS, suggesting a possible role in protein or membrane stabilizationfor this protein. Our study showed that this is also the casewith rGmD19. However, the physiological relevance of the limitedfolding promoted by SDS is unclear. We failed to detect any interactionbetween GmD19 and unilamellar liposomes made of the most abundantphospholipid found in any cell. This observation raises additionaldoubts regarding the potential for group 1 LEA proteins to engagein membrane protection via direct interaction with membrane lipids.Other researchers have proposed that the cryoprotective role ofLEA-related COR proteins (e.g. COR15a) arises from its interactionwith membrane lipids (Steponkus et al., 1998). This interaction,which alters the intrinsic curvature of the lipid monolayer ofthe inner chloroplast envelope, is mediated by the COR15am polypeptide,which is composed largely of amphipathic $alpha$ -helical regions. Incontrast, our results showed that the group 1 LEA protein assumesa largely random coil in solution and is, therefore, much lesslikely than group 2 LEA or COR15a proteins to interact with membranes.Although additional studies should be conducted to determine ifgroup 1 LEA proteins can adopt certain structures upon interactionwith other macromolecules, the evidence provided here is inconsistentwith such interactions being important for their in vivofunction.

In conclusion, we suggest that rGmD-19 can interact efficiently with water because of its hydrophilicity and the adoptionof an extended helical conformation, at very low temperatures,in combination with unordered random coil structures. Future invitro and in vivo biochemical and physicochemical analyses, includingexamination of the hydration properties of purified, recombinantrGmD-19, are under way and should provide important clues aboutthe functional roles that group 1 LEA proteins play in combatingmacromolecular destabilization because of dehydration-relatedstresses.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION RESULTS DISCUSSION MATERIALS AND METHODS LITERATURE CITED

Cloning and Expression of Soybean (Glycine max) Group 1 LEA

The soybean group 1 (GmD-19) LEA cDNA coding region (321 bp; accession nos. U66317 and AAB68027; Burns et al., 1997)was amplified using ULTma DNA polymerase (Promega, Madison, WI)and gene-specific primers containing NcoI (5'-CATGCCATGGCATCTCGTCAAAAC-3')or EcoRI (5'-CGGATTCCTCACTTATCC TGGTCTTC-3') restriction sites.The amplified fragment was digested with NcoI/EcoRI and ligatedinto the NcoI/EcoRI sites of the pET30a Escherichia coli expressionvector (Novagen, Madison, WI). His and S-tag sequences (157 bp)were then removed from the cloning vector by inverse PCR usingPfu polymerase (Life Technologies, Rockville, MD) and outward-facingprimers (5'-GGCGCGCCCTCCTTCTTAAAGTTAA-3' and 5'-GGCGCGCCATGGCATCTCGTCAAA-3')containing AscII restriction sites. The amplification productwas digested with AscII and religated with T4 ligase. The integrityof the cloned insert was confirmed by automated DNA sequencing.The resulting pET30a::D-19 was introduced into E. coli BL21 (DE3)plysS cells and grown in 2× yeast tryptone medium under kanamycinselection (50 µg mL¹) at 37°C with vigorous agitation (300 rpm). Recombinant GmD-19protein expression was induced by adding IPTG to a final concentrationof 0.1 mM when cells reached an OD₆₀₀ of 0.8. Cells were harvestedwhen the culture reached an OD₆₀₀ of 1.5. Expression of the recombinantprotein (rGmD-19) was confirmed by 15% (w/v) SDS-PAGE.

Purification of rGmD-19 from E. coli

Bacterial cells were harvested by centrifugation at 5,000g and resuspended in B-PER Bacterial Extraction buffer (Pierce, Rockford,IL) in the presence of Complete Mini protease inhibitor cocktail(Boehringer Mannheim, Indianapolis). The soluble cell lysate extractwas sonicated to reduce viscosity, heat denatured in boiling waterfor 10 min., and clarified by centrifugation at 26,500g for 20min. The clarified supernatant was concentrated using a CentriconPlus-80, MWCO 5000 polycarbonate centrifugal filter (Amicon, Beverly,MA) and dialyzed overnight against 10 mM Tris-HCl, pH 7.5, usingdialysis membrane tubing (SnakeSkin MWCO 3000, Pierce). The dialyzedextracts were subjected to preparative IEF in the presence ofampholytes (2% [v/v], pH range 5-7; Bio-Rad Laboratories, Hercules,CA) using a Rotofor Cell (Bio-Rad Laboratories) at 15-W constantpower for 4 h. Fractions were surveyed by 12% (w/v) SDS-PAGE andfractions containing rGmD-19 protein were pooled and stored at $-$ 20°C.

Further purification of the pooled IEF fractions was conducted using anionic exchange column chromatography on a High-Q column(Bio-Rad Laboratories) in 10 mM Tris-HCl, pH 7.5, eluted by a0 to 250 mM NaCl gradient at 1 mL min¹ flow rate. Collected fractions (2 mL) were analyzed by SDS-PAGE,pooled, and stored as the final purified proteins. Alternatively,rGmD-19 was purified without heat denaturation by 60% (w/v) ammoniumsulfate precipitation. Clarified supernatant was recovered anddesalted using a Centricon Plus-80, MWCO 5000 polycarbonate centrifugalfilter (Amicon) and dialyzed before preparative IEF and anion-exchangecolumn chromatography. Cation exchange column chromatography usinga High-S column (Bio-Rad Laboratories) equilibrated with 10 mMNa-acetate, pH 4.8, was used as a final purification step. rGmD-19was eluted using a 0 to 500 mM NaCl gradient at 1 mL min¹ flow rate and fractions containing the purified protein werepooled and desalted by dialysis as describedabove.

Mass Spectrometry

Molecular mass determination of rGmD-19 was performed by matrix-assisted laser-desorption ionization time of flight MS (Proflex,Bruker, Karlsruhe, Germany) using sinapinic acid as a matrix.Samples were prepared using a ZipTip_C18 reverse phase column (Millipore,Bedford, MA) following manufacturer's instructions. After desalting,samples were dissolved in 50% (v/v) acetonitrile and 0.1% (v/v)trifluoroacetic acid and then dried by gentle heating before MSanalysis. Cytochrome C (molecular mass 12,384 D) was used as acalibrationstandard.

Differential Scanning Calorimetry (DSC) and Thermal Analysis

Three milligrams of lyophilized protein powder was weighed on a DSC volatile samples pan and hydrated under 80% (v/v) relativehumidity controlled by saturated KNO₃ at room temperature. Thermalevents were measured from 0°C to 100°C at a rate of 10°C min¹ using a Differential Scanning Calorimeter DSC-4 and DSC-7 (Perkin-Elmer,Norwalk, CT) calibrated for temperature using methylene chloride( $-$ 95°C) and indium (156°C) standards and for energy with indium(28.54 Jg¹) as previously described (Leprince and Vertucci, 1995). Heliumgas was used for purging at a rate of 20 mL min¹. To standardize the dry mass of each sample, heat flow in everyDSC scan was divided by the sample dryweight.

UV Absorption Spectroscopy

UV absorption spectra were recorded with an HP 8453 diode array spectrophotometer (Hewlett-Packard, St. Paul). The concentrationof rGmD-19 was calculated from the absorbance of the samples at280 nm in the presence of 6 M guanidinium-HCl ( $epsilon$ _Tyr = 1, 285 cm^1
M1; Pace et al., 1995). Second derivatives were calculated by theSavitzky-Golay differentiation technique using a filtering lengthof 9. The temperature dependence of the difference between thesecond derivatives at 283 and 279 nm was determined in 50 m[scap]mphosphate buffer solutions. The sample temperature was modifiedand controlled by a Peltier temperature-controlled cellholder.

CD Analysis

CD spectra were acquired with a CD spectropolarimeter (model J715, Jasco, Easton, MD) using a 0.1-cm path-length cell overthe 184- to 260-nm range. The temperature was controlled by acirculating water bath (model RTE 111, Neslab, Newington, NH)and determined directly into the cell using a thermocouple. CDspectra were acquired every 1 nm with 2 s averaging time per pointand a 1-nm band-pass. Quadruplicate average spectra were correctedfor the blank and smoothed. CD data were expressed as mean residueellipticity values and analyzed by the method of Sreerama et al.(1999).

	ACKNOWLEDGMENTS

We thank Sue Ann Hudiburg and Janet Rogers at the Oklahoma State University Recombinant DNA/Protein Resource Facility (Stillwater,OK) for the synthesis of oligonucleotides and automated DNA sequencingservices. We also thank Dr. David Quilici at the Mass SpectrometryFacility at the University of Nevada (Reno) for providing massspectrometrydata.

	FOOTNOTES

Received June 15, 2001; returned for revision September 19, 2001; accepted November 3, 2001.

¹ This work was supported by the United States Department of Agriculture, National Research Initiative-Competitive Grant Program(grant no. 99-35100-7004 to J.C.C.), by the National Institutesof Health (grant no. GM 55622 to J.L.S.), and by the Oklahomaand Nevada Agricultural Experiment Stations. The materials describedin this manuscript will be distributed publicly upon request bycontacting the correspondingauthor.

² Present address: 193 E.R. Madigan Laboratory, 1201 W. Gregory Avenue, Urbana, IL61801.

^* Corresponding author; e-mail jcushman{at}unr.edu; fax 775-784-1650.

Article, publication date, and citation information can be found at www.plantphysiol.org/cgi/doi/10.1104/pp.010521.

LITERATURE CITED

TOP
ABSTRACT
INTRODUCTION
RESULTS
DISCUSSION
MATERIALS AND METHODS
LITERATURE CITED

Adzhubei AA, Sternberg MJE (1993) Left-handed polyproline II helices commonly occur in globular proteins. J Mol Biol 229: 472-493[CrossRef][ISI][Medline]
Baker J, Steele C, Dure L III (1988) Sequence and characterization of 6 Lea proteins and their genes from cotton. Plant Mol Biol 11: 277-291[CrossRef][ISI]
Bartels D, Singh M, Salamini F (1988) Onset of desiccation tolerance during development of the barley embryo. Planta 175: 485-492[CrossRef]
Bray EA (1997) Plant responses to water deficit. Trends Plant Sci 2: 48-54
Burns WC, Maitra N, Cushman JC (1997) Isolation and characterization of a cDNA encoding a group I LEA protein from soybean (accession no. U66317) PGR97-016. Plant Physiol 113: 663[CrossRef][Medline]
Bush CA, Ralapati S, Matson GM, Yamasaki RB, Osuga DT, Yeh Y, Feeney RE (1984) Conformation of the antifreeze glycoprotein of polar fish. Arch Biochem Biophys 232: 624-631[CrossRef][Medline]
Chandler PM, Robertson M (1994) Gene expression regulated by abscisic acid and its relation to stress tolerance. Annu Rev Plant Physiol Plant Mol Biol 45: 113-141[CrossRef][ISI]
Close TJ (1996) Dehydrins: emergence of a biochemical role of a family of plant dehydration proteins. Physiol Plant 97: 795-803[CrossRef]
Close TJ (1997) Dehydrins: a commonalty in the response of plants to dehydration and low temperature. Physiol Plant 100: 291-296[CrossRef]
Creamer TP (1998) Left-handed polyproline II helix formation is (very) locally driven. Protein Struct Funct Genet 33: 218-226
Crowe JH, Hoekstra FA, Crowe LM (1992) Anhydrobiosis. Ann Rev Physiol 54: 570-599
Cuming AC (1999) LEA proteins. In PR Shewry, R Casey, eds, Seed Proteins. Kluwer Academic Publishers, Dordrecht, The Netherlands, pp 753-780
Danyluk J, Perron A, Houde M, Limin A, Fowler B, Benhamou N, Sarhan F (1998) Accumulation of an acidic dehydrin in the vicinity of the plasma membrane during cold acclimation of wheat. Plant Cell 10: 623-638[Abstract/Free Full Text]
Davies PL, Sykes BD (1997) Antifreeze proteins. Curr Opin Struct Biol 7: 828-834[CrossRef][ISI][Medline]
Demchenko AP (1986) Fluorescence analysis of protein dynamics. Essays Biochem 22: 120-157[ISI][Medline]
Dure L III (1993a) Structural motifs in LEA proteins. In TJ Close, EA Bray, eds, Plant Responses to Cellular Dehydration during Environmental Stress. American Society of Plant Physiologists, Rockville, MD, pp 91-103
Dure L III (1993b) A repeating 11-mer amino acid motifs and plant desiccation. Plant J 3: 363-369[CrossRef][ISI][Medline]
Dure L III (1997) LEA proteins and the desiccation tolerance of seeds. Cell Mol Biol Plant Seed Dev 4: 525-543
Dure L III, Crouch M, Harada J, Ho THD, Mundy J, Quatrano R, Thomas T, Sung ZR (1989) Common amino acid sequence domains among the LEA proteins of higher plants. Plant Mol Biol 12: 475-486[CrossRef][ISI]
Eom J, Baker WR, Kintanar A, Wurtele ES (1996) The embryo-specific EMB-1 protein of Daucus carota is flexible and unstructured in solution. Plant Sci 115: 17-24[CrossRef]
Esperlund M, Saeboe-Larssen S, Hughes DW, Galau GA, Larsen F, Jakobsen KS (1992) Late embryogenesis abundant genes encoding proteins with different numbers of hydrophobic repeats are regulated differentially by abscisic acid and osmotic stress. Plant J 2: 241-252[ISI][Medline]
Garay-Arroyo A, Colmenero-Flores JM, Garciarrubio A, Covarrubias AA (2000) Highly hydrophilic proteins in prokaryotes and eukaryotes are common during conditions of water deficit. J Biol Chem 275: 5668-5674[Abstract/Free Full Text]
Houde M, Daniel C, Lachapella M, Allard F, Lalibertee J, Sarhan F (1995) Immunolocalization of freezing-tolerance associated proteins in the cytoplasm and nucleoplasm of wheat crown tissue. Plant J 8: 583-593[CrossRef][ISI][Medline]
Hughes DW, Galau GA (1989) Temporally modular gene expression during cotyledon development. Genes Dev 3: 358-369[Abstract/Free Full Text]
Imai T, Chang L, Ohta A, Bray E, Takagi M (1996) A lea-class gene of tomato confers salt and freezing tolerance when expressed in Saccharomyces cerevisiae. Gene 170: 243-248[CrossRef][ISI][Medline]
Ingram J, Bartels D (1996) The molecular basis of dehydration tolerance in plants. Annu Rev Plant Physiol Plant Mol Biol 47: 377-403[CrossRef][ISI][Medline]
Ismail AM, Hall AE, Close TJ (1999) Purification and partial characterization of a dehydrin involved in chilling tolerance during seedling emergence of cowpea. Plant Physiol 120: 237-244[Abstract/Free Full Text]
Lane AN, Hays LM, Feeney RE, Crow LM, Crowe JH (1998) Conformational and dynamic properties of a 14 residue antifreeze glycoprotein from Antarctic cod. Protein Sci 7: 1555-1563[Abstract]
Lane AN, Hays LM, Tsvetkova N, Feeney RE, Crowe LM, Crowe JH (2000) Comparison of the solution conformation and dynamics of antifreeze glycoproteins from Antarctic fish. Biophys J 78: 3195-3207[Abstract/Free Full Text]
Leprince O, Vertucci CW (1995) A calorimetric study of the glass transition behaviors in axes of bean seeds with relevance to storage stability. Plant Physiol 109: 1471-1481[Abstract]
Lisse T, Bartels D, Kalbitzer HR, Jaenicke R (1996) The recombinant dehydrin-like desiccation stress protein from the resurrection plant Craterostigma plantagineum displays no defined three-dimensional structure in its native state. Biol Chem 377: 555-561[ISI][Medline]
McCubbin WD, Kay CM, Lane BG (1985) Hydrodynamic and optical properties of the wheat germ Em protein. Can J. Biochem Cell Biol 63: 803-811
Moons A, Bauw G, Prinsen E, Van Montagu M, Straeten DVD (1995) Molecular ad physiological responses to abscisic acid and salts in roots of salt-sensitive and salt-tolerant Indica rice varieties. Plant Physiol 107: 177-186[Abstract]
Nylander M, Svensson J, Palva ET, Welin BV (2001) Stress-induced accumulation and tissue-specific localization of dehydrins in Arabidopsis thaliana. Plant Mol Biol 45: 263-279[CrossRef][ISI][Medline]
Pace NC, Vadjos F, Fee L, Grimsley G, Gray T (1995) How to measure and predict the molar absorption coefficient of a protein. Protein Sci 4: 2411-2423[Abstract]
Park SH, Shalongo W, Stellwagen E (1997) The role of PII conformations in the calculation of peptide fractional helix content. Protein Sci 6: 1694-1700[Abstract]
Ragone R, Colonna G, Balestrieri C, Servillo L, Irace G (1984) Determination of tyrosine exposure in proteins by second-derivative spectroscopy. Biochemistry 23: 1871-1875[CrossRef][Medline]
Reid JL, Walker-Simmons MK (1993) Group 3 late embryogenesis abundant proteins in desiccation-tolerant seedlings of wheat (Triticum aestivum L.). Plant Physiol 102: 125-131[Abstract]
Roberts JK, Noelle AD, Wilma LL, Dure L III (1993) Cellular concentrations and uniformity of cell-type accumulation of two lea proteins in cotton embryos. Plant Cell 5: 769-780[Abstract/Free Full Text]
Russouw PS, Farrant J, Brandt W, Lindsey GG (1997) The most prevalent protein in a heat-treated extract of pea (Pisum sativum) embryos is an LEA group I protein; its conformation is not affected by exposure to high temperature. Seed Sci Res 7: 117-123
Siermala M, Juhola M, Vihinen M (2000) Neural network prediction of polyproline type II secondary stuctures. Stud Health Technol Inform 77: 475-479[Medline]
Soulages JL, Bendavid O (1998) The lipid binding activity of the exchangeable apolipoprotein apolipophorin-III correlated with the formation of a partially folded conformation. Biochemistry 37: 10203-10210[CrossRef][Medline]
Sreerama N, Vanyaminov SY, Woody RW (1999) Estimation of the number of $alpha$ -helical and $beta$ -strand segments in proteins using circular dichroism spectroscopy. Protein Sci 8: 370-380[Abstract]
Stacy RAP, Aalen RB (1998) Identification of sequences homology between the internal hydrophilic repeated motifs of group 1 late-embryogenesis-abundant proteins in plants and hydrophilic repeats of the general stress protein GsiB of Bacillus subtilis. Planta 206: 476-478[CrossRef][ISI][Medline]
Stapley BJ, Creamer TP (1999) A survey of left-handed polyproline II helices. Protein Sci 8: 587-595[Abstract]
Steponkus PL, Uemura M, Joseph RA, Gilmour SJ, Thomashow MF (1998) Mode of action of the COR15a gene of the freezing tolerance of Arabidopsis thaliana. Proc Natl Acad Sci 95: 14570-14575[Abstract/Free Full Text]
Swire-Clark GA, Marcotte WR (1999) The wheat LEA protein Em functions as a osmoprotective molecule in Saccahromyces cerevisiae. Plant Mol Biol 39: 117-128[CrossRef][ISI][Medline]
Thomashow MF (1998) Role of cold-responsive genes in plant freezing tolerance. Plant Physiol 118: 1-17[Free Full Text]
Tomczak MM, Hincha DK, Estrada SD, Feeney RE, Crowe JH (2001) Antifreeze proteins differentially affect model membranes during freezing. Biochim Biophys Acta 1511: 255-263[Medline]
Uemura M, Gilmour SJ, Thomashow MF, Steponkus PL (1996) Effects of COR6.6 and COR15am polypeptides encoded by COR (cold-regulated) genes of Arabidopsis thaliana on the freeze-induced fusion and leakage of liposomes. Plant Physiol 111: 313-327[Abstract]
van Zee K, Chen FQ, Hayes PM, Close TJ, Chen THH (1995) Cold-specific induction of a dehydrin gene family member in barley. Plant Physiol 108: 1233-1239[Abstract]
Völker U, Engelmann S, Maul B, Riethdorf S, Völker A, Schmid R, Mach H, Hecker M (1994) Analysis of the induction of general stress proteins of Bacillus subtilis. Microbiology 140: 741-752[Abstract]
Walters C, Ried JL, Walker-Simmons MK (1997) Heat-soluble proteins extracted from wheat embryo have tightly bound sugars and unusual hydration properties. Seed Sci Res 7: 125-134
Webb MS, Gilmour SJ, Thomashow MF, Steponkus PL (1996) Effects of COR6.6 and COR15am polypeptides encoded by COR (cold-regulated) genes of Arabidopsis thaliana on dehydration-induced phase transitions of phospholipid membranes. Plant Physiol 111: 301-312[Abstract]
Whitsitt MS, Collins RG, Mullet JE (1997) Modulation of dehydration tolerance in soybean seedlings. Plant Physiol 114: 917-925[Abstract]
Woody RW (1992) Circular dichroism and conformation of unordered polypeptides. Adv Biophys Chem 2: 37-79
Xu D, Duan X, Wang B, Hong B, Ho TH, Wu R (1996) Expression of a late embryogenesis abundant protein gene, HVA1, from barley confers tolerance to water deficit and salt stress in transgenic rice. Plant Physiol 110: 249-257[Abstract]
Yeh T, Feeney RE (1996) Antifreeze proteins: structures and mechanisms of function. Chem Rev 96: 601-618[CrossRef][ISI][Medline]
Zhang L, Ohta A, Takagi M, Imai R (2000) Expression of plant group 2 and group 3 lea genes in Saccharomyces cerevisiae revealed functional divergence among LEA protein. J Biochem 127: 611-616[Abstract/Free Full Text]

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Temperature-Induced Extended Helix/Random Coil Transitions in a Group 1 Late Embryogenesis-Abundant Protein from Soybean1

Temperature-Induced Extended Helix/Random Coil Transitions in a Group 1 Late Embryogenesis-Abundant Protein from Soybean¹