The Role of N and C Termini in the Antifreeze Activity of Winter Flounder (Pleuronectes americanus) Antifreeze Proteins*

Woon-Kai LowDagger §, Qingsong LinDagger ||**, and Choy L. HewDagger §||**DaggerDagger

From the Dagger  Division of Structural Biology and Biochemistry, Hospital for Sick Children, Toronto, Ontario M5G 1X8, Canada, the § Department of Biochemistry and || Department of Laboratory Medicine and Pathobiology, University of Toronto, Toronto, Ontario M5G 1L5, Canada, and the ** Department of Biological Sciences, National University of Singapore, Singapore 119 260, Singapore

Received for publication, January 5, 2003

    ABSTRACT
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Antifreeze proteins (AFPs) are found in many marine fish and have been classified into five biochemical classes: AFP types I-IV and the antifreeze glycoproteins. Type I AFPs are alpha -helical, partially amphipathic, Ala-rich polypeptides. The winter flounder (Pleuronectes americanus) produces two type I AFP subclasses, the liver-type AFPs (wflAFPs) and the skin-type AFPs (wfsAFPs), that are encoded by distinct gene families with different tissue-specific expression. wfsAFPs and wflAFPs share a high level of identity even though the wfsAFPs have approximately half the activity of the wflAFPs. Synthetic polypeptides based on two representative wflAFPs and wfsAFPs were generated to examine the role of the termini in antifreeze activity. Through systematic exchange of N and C termini between wflAFP-6 and wfsAFP-2, the termini were determined to be the major causative agents for the variation in activity levels between the two AFPs. Furthermore, the termini of wflAFP-6 possessed greater helix-stabilizing ability compared with their wfsAFP-2 counterparts. The observed 50% difference in activity between wflAFP-6 and wfsAFP-2 can be divided into ~20% for differences at each termini and ~10% for differences in the core. Furthermore, the N terminus was determined to be the most critical component for antifreeze activity.

    INTRODUCTION
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Fish antifreeze proteins are diverse in structure and have been grouped into five biochemical classes based on their structural characteristics: antifreeze proteins (AFPs)1 types I-IV and antifreeze glycoproteins (AFGPs) (1-3). Although diverse in structure, all AF(G)Ps act by what is known as the adsorption inhibition mechanism (2, 4-6), where the AF(G)Ps lower the observed freezing point in a non-colligative manner creating a hysteresis between the equilibrium melting point and the observed freezing point. The degree of thermal hysteresis is used as a measure of AF(G)P activity.

Type I AFPs are Ala-rich, partially amphipathic single alpha -helical polypeptides found in several sculpins and righteye flounders (2, 7, 8). The winter flounder (Pleuronectes americanus) produces two subclasses of type I AFPs, the liver-type (wflAFPs) and the skin-type AFPs (wfsAFPs), which are encoded by distinct gene families (9). wflAFP-6 (formerly known as HPLC-6) is the major winter flounder plasma AFP and is produced in the liver as a prepro-precursor, and then secreted into circulation, where it is then processed into the mature polypeptide of 37 residues (10, 11). Conversely, the wfsAFPs have a wider tissue distribution and are produced as mature intracellular polypeptides (9).

The wflAFPs and wfsAFPs share a high level of structural identity even though the wfsAFPs have approximately half the activity of wflAFP-6 (9). Both wflAFPs and wfsAFPs possess two 11-residue motifs of the structure TaaXAXXAAXX (where the first Thr is always conserved, uppercase A is a conserved Ala, lowercase a is almost always Ala, and X can be one of several amino acids), with wflAFP-6 having a third full motif at the N terminus (see Fig. 1). Furthermore, the wflAFPs possess complete ice-binding motifs (IBMs), LTAAN (8), whereas the wfsAFPs have incomplete IBMs of the form ATAAA, and this difference in IBMs has been proposed to be the cause of the lower thermal hysteresis found in wfsAFPs (12). However, the introduction of two proposed IBMs (KT-D, and DT-K) into wfsAFP-2 did not produce any improvement in activity (12). Furthermore, the introduction of the LTAAN IBM into wfsAFP-2 only increased the activity by ~15%, yet lowered the helical content from 80 to 60%.2

The IBM hypothesis is based on earlier beliefs that wflAFP-6 requires regularly spaced polar groups to match the arrangement of water molecules on the ice surface for the formation of hydrogen bonds (5, 13-16). However, recent study of wflAFP-6 has suggested that the major ice-binding surface resides on the hydrophobic face of the polypeptide, with major contribution from conserved Ala residues. Furthermore, the driving forces behind ice binding are van der Waals interactions and the hydrophobic effect (17-21). The major sequence variations between wflAFP-6 and the wfsAFPs are in the N and C termini (see Fig. 1). Most notably, wflAFP-6 has the N-terminal sequence DTASDA, whereas all wfsAFPs begin with MDAP (9). Furthermore, the MDAP sequence can be found in the longhorn sculpin skin-type AFP (22), and in the minor serum AFPs of the shorthorn and grubby sculpins (23, 24), all of which have ~50% activity of wflAFP-6. The region of highest variability in type I AFPs lies in the C-terminal regions (7, 9).

This study examines the contributions of the N- and C-terminal sequences to the antifreeze activity of the liver- and skin-type AFPs. Polypeptides were synthesized where the N- and C-terminal sequences of two representative AFPs, wflAFP-6 and wfsAFP-2, were systematically exchanged, then assayed for antifreeze activity and alpha -helical content. The results demonstrated that the difference in activity was caused primarily by sequence variations at the N and C termini. Furthermore, the N and C termini of wflAFP-6 were able to confer higher overall helical content and greater thermal stability over their skin-type AFP counterparts.

    EXPERIMENTAL PROCEDURES
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Polypeptide Synthesis and Purification-- Polypeptides were synthesized by continuous flow Fmoc chemistry on NovaSyn KA 100 resin (25) using a Biolynx 4170 automated peptide synthesizer (Amersham Biosciences, Montreal, Quebec, Canada) by the Advanced Protein Technology Centre, Hospital for Sick Children (Toronto, Ontario, Canada). A 20% piperidine solution in dimethyl formamide was used for removal of the Fmoc protection group. For each gram of resin (0.1 nmol substitution), a 4× excess of Fmoc amino acid activated with O-(7-azabenzotriazol-1-yl)-N,N,N',N'-tetramethyluronium hexafluorophosphate and diisopropylethylamine (1:1:2, mol/mol/mol) (26) was used for the coupling reaction, with a reaction time of 1 h. Peptide-resin conjugates were washed with dimethyl formamide, diethyl ether, and dried under reduced pressure. Dry peptide-resin conjugates were cleaved with 20 ml of trifluoroacetic acid containing 4 ml of thioanisole, 0.4 ml of m-cresol, 2 ml of 1,2-ethanedithiol, 3 ml of ethylmethylsulfide, and 4 ml of bromotrimethylsilane at 0 °C for 1 h. Peptides were extracted, dissolved in 0.1% trifluoroacetic acid, and desalted on a Sephadex G10 column. Crude polypeptide preparations were further purified by reverse-phase HPLC using a Jupiter 10-µm C4 300 Å (250 mm × 21.20 mm) column (Phenomenex, Torrance, CA) using an acetonitrile gradient in 0.1% trifluoroacetic acid. Homogeneity of peptides was analyzed by C18 reverse-phase HPLC, amino acid analysis, and electrospray ionization mass spectrometry. All polypeptides were synthesized with free N termini and amidated C termini except where indicated.

Measurement of Antifreeze Activity-- Synthetic polypeptides were assayed for antifreeze activity using a Clifton Nanolitre Osmometer (Clifton Technical Physics, Hartford, NY) as previously described (27). Briefly, purified and lyophilized polypeptides were re-dissolved in 0.1 M ammonium bicarbonate (pH 7.9). Serial dilutions were made for each polypeptide and thermal hysteresis readings taken for each dilution. Measurements at each dilution were averaged from readings from four to six different wells in the sample plate. Concentration was determined by amino acid analysis on the two highest diluted samples. Amino acid analysis was performed by the Advanced Protein Technology Centre, Hospital for Sick Children. Percentage of activity was determined by comparison of thermal hysteresis values for each polypeptide at concentrations of 0.5-3 mM at intervals of 0.5 mM, and error bars represent ±1 standard deviation of the average percent activity reported. From results obtained for Skin(wt), results from different assay groups were reproducible with a 5% experimental error.

Circular Dichroism Spectroscopy-- Circular dichroism spectroscopy was performed using an AVIV 62A DS circular dichroism spectrometer (AVIV Instruments, Inc., Lakewood, NJ) equipped with a thermal control unit in a 1-mm quartz cuvette. Polypeptides were dissolved in 0.1 M ammonium bicarbonate (pH 7.9), and assayed at two concentrations in the range of 10 or 50 µM. Spectra were collected with 1-nm bandwidth and 1 nm between data points at 0 and 40 °C using an averaging time of 6 s from 250 to 190 nm. Thermal denaturation was performed using the same parameters at 222 nm with temperature equilibrium time of 30 s/°C. All spectra were the result of subtraction of data collected on 0.1 M ammonium bicarbonate alone. The fraction helix (fH) for each polypeptide at indicated temperatures was calculated by the method of Luo and Baldwin (28) from mean molar residue ellipticity observed at 222 nm (q222) using Equation 1.


f<SUB><UP>H</UP></SUB><UP> = </UP><FR><NU>(<UP>&thgr;<SUB>222</SUB> − &thgr;<SUB>C</SUB></UP>)</NU><DE>(<UP>&thgr;<SUB>H</SUB> − &thgr;<SUB>C</SUB></UP>)</DE></FR> (Eq. 1)
Temperature and chain length dependences of theta C and theta H in Equation 1 are defined by Equations 2 and 3.
&thgr;<SUB><UP>C</UP></SUB><UP> = 2220 − 53</UP>T (Eq. 2)

&thgr;<SUB><UP>H</UP></SUB><UP> = </UP>(<UP>−44,000 + 250</UP>T)(1−3/N<SUB>r</SUB>) (Eq. 3)
T is the temperature in °C, and Nr is the chain length in residues. Where data are presented as percentages, fH was multiplied by 100. Values reported at 0 °C are averages of three to five independent readings.

Pairwise Comparison (Table I)-- In column 1 of Table I, the percentage of activity of the polypeptide containing the wfsAFP-2 region was subtracted from the value for the polypeptide containing the wflAFP-6 region. Positive values indicate higher activity in the presence of wflAFP-6 components, and negative values indicate higher activity for the wfsAFP-2 components. Each column 1 value was assigned a label: A1-A4, B1-B4, and C1-C4. In column 3, an analysis similar to that in column 1 was performed on the helical contents for each analogue, with each resulting value assigned labels a1-a4, b1-b4, and c1-c4. Statistical analysis of the data was achieved by performing standard t tests assuming equal variances between the two mean values obtained from the activity levels determined from 0.5 to 3 mM at intervals of 0.5 mM after normalization to the activity level of Liver(wt). An alpha  value of 0.05 and a null hypothesis of no difference between the indicated mean values were used.

Pairwise Analysis of the Increased Activity of wflAFP-6 Components and the Dependence on the Characteristics of the Remainder of the Polypeptide (Table II)-- In Table II, the values in each column were the result of the calculation shown. For example, in column 1, row A, the A1 value was derived from the difference in activity when [S]-Nterm was replaced by [L]-Nterm (A1 value, Table I) with the remaining components composed of wflAFP-6 components. The A3 value was derived from the difference in activity when the same exchange was performed, but with wfsAFP-2 components comprising the remainder of the polypeptide. Thus, the first value presented in Table II, column 1, row A is the difference between the increased activity associated with the replacement of [S]-Nterm by [L]-Nterm when the remainder of the polypeptide was composed of wflAFP-6 components as opposed to wfsAFP-2 components. All other values determined in Table II follow the same methodology. Statistical analysis was performed as described for Table I.

    RESULTS
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

A comparison of wflAFP-6 and wfsAFP-2 sequences demonstrated that the region of highest identity between the two polypeptides occurs in the central region (wflAFP-6 core; L-core and wfsAFP-2 core; S-core), with no identity at the termini (see Fig. 1A). For wflAFP-6, the N-terminal sequence, [L]-Nterm, was defined as DTASDA, and the C-terminal sequence, [L]-Cterm, was defined as AR. Correspondingly, in wfsAFP-2, the N-terminal sequence, [S]-Nterm, was defined as MDAP, and C-terminal sequence, [S]-Cterm, defined as KAGAAR.


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Fig. 1.   Synthetic polypeptide analogues of wflAFP-6 and wfsAFP-2 used to determine the role of N and C termini in antifreeze activity. All polypeptides were synthesized with free N termini, and amidated C termini except where indicated by -OOH. The putative Asp-2/Lys-6 (D2-K6) salt bridge (see "Discussion") is indicated by double-arrowhead lines. IBMs are indicated with the complete IBM of wflAFP-6 (LTAAN) indicated above its sequence, and the incomplete IBM of wfsAFP-2 (ATAAA) indicated below its sequence. A, wild-type wflAFP-6 and wfsAFP-2 sequences. wflAFP-6 sequence is in uppercase text, whereas wfsAFP-2 sequence is in lowercase text. The polypeptides were divided into three regions: N terminus, core region, and C terminus. Identical residues between wflAFP-6 and wfsAFP-2 are highlighted in gray. Corresponding wflAFP-6 and wfsAFP-2 N and C termini are indicated. B, sequence of polypeptide analogues. The wflAFP-6 analogue is designated Liver(wt), and the wfsAFP-2 analogue is designated Skin(wt). Uppercase and lowercase notation is maintained to distinguish the original source of each region of the polypeptides.

The synthetic polypeptides were designed to examine the effects of N-terminal exchange, C-terminal exchange, and simultaneous exchange of both termini. In the N-terminal exchange series, polypeptides consisting of wild-type sequences for wfsAFP-2 and wflAFP-6, Skin(wt) and Liver(wt), were also assayed. The Skin(wt) activity was ~50% of Liver(wt) (Fig. 2D), in agreement with previous results (9). For ease of comparison, all activity levels were expressed as a percentage of Liver(wt) activity. Skin(wt) was used as an internal control to allow comparison of results between the three groups of polypeptides. Fig. 2D summarizes the observed activity levels for each polypeptide, and Table I (column 1) details the difference in activity between polypeptides that varied at a single region. In each instance (Table I, column 1) differences in activity levels were determined to be statistically significant.


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Fig. 2.   Thermal hysteresis levels of the synthetic polypeptides. All data point error bars are ±1 standard deviation. A, results of N-terminal exchange. Thermal hysteresis levels of Liver(wt) and Skin(wt) were assayed in this group. B, results of C-terminal exchange. Skin(wt) control and Liver(wt) control refer to data points collected in A. C, results of simultaneous exchange of N and C termini. Skin(wt) control and Liver(wt) control refer to data points collected in A. D, activity of each polypeptide expressed as a percentage of Liver(wt).


                              
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Table I
Pairwise comparison of the activity and helical contents of polypeptides differing at a single region
The resulting values of column 1 were assigned labels (A1 to A4, B1 to B4, and C1 to C4) for use in the analysis presented in Table II. The * indicates data in column 4 containing Skin[L] data. For the statistical analysis: H0 = no difference between means, alpha  = 0.05, and failure to reject the null hypothesis (H0) is indicated by gray highlights. For column 5 in A and B, averages are derived from values in column 3 without inclusion of data containing Skin[L]. For column 6 in c, averages are from the indicated values of column 3.

The Exchange of N- or C-terminal Sequences-- Lack of C-terminal amidation in the wfsAFP-2 C terminus ([L]Skin-OOH) did not significantly affect activity (Fig. 2A). The conversion of the wflAFP-6 N or C terminus to the corresponding wfsAFP-2 sequences resulted in a loss of ~27% of activity (Fig. 2D; Table I, column 1, values A1 and C1). In wfsAFP-2, replacement of the N or C terminus with those found in wflAFP-6 resulted in a gain of ~15% in activity (Fig. 2D; Table I, column 1, values A3 and C3).

When [S]-Nterm was replaced by [L]-Nterm, the magnitude of the increased activity was ~14% greater when the remaining polypeptide contained L-core and [L]-Cterm (Table II, column 1, A1-A3 value). When the remaining polypeptide was composed of a mixture of components, the increase in activity associated with the same exchange was ~4% higher in the presence of S-core and [L]-Cterm as opposed to L-core and [S]-Cterm (Table II, column 1, A4-A2 value). Similarly, for the exchange of [S]-Cterm with [L]-Cterm, the increased activity was ~11% higher when wflAFP-6 components were present (Table II, column 1, C1-C3 value). Furthermore, the increased activity associated with this exchange was ~7% higher when [L]-Nterm and S-core were present as opposed to the opposite composition (Table II, column 1, C4-C2 value).


                              
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Table II
Pairwise analysis of the increased activity of a wflAFP-6 component and the dependence on the characteristics of the remainder of the polypeptide
All values (A1 to A4, B1 to B4, and C1 to C4) are derived in Table I. In the three letter notation, X is the site of exchange, and core regions are abbreviated to single letters. The values obtained in on the right of each column are derived from the calculations shown on the left. For statistical analysis: H0 = no difference between means, alpha  = 0.05, and failure to reject the null hypothesis is indicated by gray highlighting.

Simultaneous Exchange of N- and C-terminal Sequences-- The [L]Skin[L] polypeptide was similar to a previously studied wflAFP-6 mutation, ATAAA, which was reported to have ~85% of the activity of a wild-type analogue as determined by the activity curves presented by Loewen et al. (29). The ATAAA analogue differed from [L]Skin[L] at positions 8 and 30, where ATAAA possessed Ala instead of Lys. Loewen et al. (29) observed lowered solubility for ATAAA, which affected their analysis of the analogue; however, no solubility issues were observed with [L]Skin[L] for the concentrations used here. If the experimental error of ~5% between assays is considered, then the combined effects of N- and C-terminal exchange on thermal hysteresis levels appeared to be somewhat additive. For [L]Skin and Skin[L], activity was increased in each case to ~64%, and ~67% of Liver(wt) (Fig. 2D). In combination, the exchange of both N- and C-terminal sequences, [L]Skin[L], resulted in activity of ~89%. Similarly, the 54% level of activity for [S]Liver[S] was close to the level of activity expected from the combined reductions for each individual exchange.

The simultaneous exchange of both termini was also evaluated as a single exchange in the core region. Thus, replacement of L-core in wflAFP-6 with S-core (essentially a replacement of complete IBMs with incomplete IBMs) resulted in a loss of ~11% of activity (Table I, column 1, value B1). The corresponding exchange in wfsAFP-2 resulted in a gain of ~3% in activity (Table I, column 1, value B3). The magnitude of the effect of the S-core to L-core exchange was greater by ~7% in the context of the wflAFP-6 termini than for the wfsAFP-2 termini (Table II, column 1, B1-B3 value). In the mixed-termini case, the magnitude of the exchange was more prominent by ~3% when the termini were composed of [L]-Nterm and [S]-Cterm then when composed of [S]-Nterm and [L]-Cterm (Table II, column 1, B4-B2 value).

Pairwise Comparison of the Effects of the N Terminus, Core Region, and C Terminus on Antifreeze Activity-- A pairwise comparison of activity levels between polypeptides that differed at a single region was performed to address the experimental error involved in each individual assay. Each region of wflAFP-6 demonstrated a higher level of activity than the corresponding region of wfsAFP-2. The [L]-Nterm provided an average improvement of ~20% (± 6%), L-core an improvement of ~7% (± 4%), and [L]-Cterm an improvement of ~22% (± 5%) in activity over the corresponding wfsAFP-2 components (Table I, column 1). Only in the evaluation of the core region did the error significantly impact the average value determined; nevertheless, the general trend was toward higher activity when the L-core was present as opposed to the S-core. However, as demonstrated in Table II, the magnitude of the increased activity associated with a wflAFP-6 region over that of the corresponding wfsAFP-2 region was dependent on the identities of the remaining regions.

The Magnitude of the Increase in Activity Associated with a wflAFP-6 Component Is Dependent on the Identity of the Remaining Regions-- In Table II (columns 3 and 5), a comparison of the values in Table I (column 1) was performed to determine the impact of the identities of the other regions that were present during the three exchanges. The presence of [L]-Cterm during exchange at the N terminus produced a ~9% higher improvement of activity compared with when the [S]-Cterm was present (Table II, column 3, A), and a ~5% higher improvement of activity was observed in the presence of L-core compared with S-core (Table II, column 5, A). Thus, a 4% higher improvement of activity (Ax1-Ax2 value) was observed when the wflAFP-6 component was present at the C terminus compared with when it was present within the core. Similarly, the improved activity of L-core over S-core demonstrated a 5% higher increase in the presence of [L]-Nterm over [S]-Nterm (Table II, column 3, B). For this same exchange, a slightly higher increase in activity was noted in the presence of [L]-Cterm when [S]-Nterm was present. However, the observed increase in activity when [L]-Nterm was present was not statistically significant (Table II, column 6, B). In this exchange, the improvement of activity associated with L-core was higher when wflAFP-6 components were present at the N terminus as compared with when they were present at the C terminus (Bx1-Bx2 value). The improvement of activity with [L]-Cterm in place of [S]-Cterm demonstrated a 9% higher enhancement in the presence of [L]-Nterm (Table II, column 5, C). For this exchange, the increased difference in activity levels when L-core was present was not statistically significant when [L]-Nterm was also present; however, the result was significant in the presence of [S]-Nterm (Table II, column 6, C). For this exchange, the improvement in activity was higher when wflAFP-6 components were present at the N terminus compared with when they were present in the core (Cx1-Cx2 value). All trends indicated that the improvement of activity associated with each wflAFP-6 component was always greater when other regions of wflAFP-6 were present. Furthermore, the location of the other wflAFP-6 components demonstrated differing levels of influence on the increased activity associated with each exchange, with the order of dependence for other regions being N terminus > C terminus > core. This order of dependence was also apparent in the values determined in column 1 (Table II). For example, in the A4-A2 value (Table II, column 1, A), the degree of activity enhancement was higher for the S-core and [L]-Cterm combination than for L-core and [S]-Cterm because the effect of the C terminus took precedence. This dependence appeared to have a "long range" effect, as the increased activity associated with [L]-Nterm over [S]-Nterm was more dependent on the identity of the opposite terminus, not the core region that was adjacent to it. The dependence of activity levels on the identity of the opposite terminus was also observed with the C terminus exchange.

alpha -Helical Content of Polypeptides at 0 °C-- Each polypeptide was assayed for its alpha -helical content utilizing circular dichroism (CD) spectroscopy. Spectra (data not shown) were recorded at 0 and 40 °C in 0.1 M ammonium bicarbonate (pH 7.9) at two different concentrations. At 0 °C, all polypeptides displayed spectra indicative of high alpha -helical content with typical negative minima at 222 and 208 nm, and positive maximums at approximately 192 nm. At 40 °C, the spectra were indicative of helix-random coil mixed structures and were identical at two different concentrations. Helical content determinations indicated Liver(wt) to be nearly entirely alpha -helical (~95%), which was in good agreement with previous structural studies of wflAFP-6 (8, 30, 31), and Skin(wt) was found to have a helical content of ~82% (Fig. 3).


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Fig. 3.   alpha -helical content and thermal denaturation (unfolding) of the synthetic polypeptides. A fraction helix (fH) value of 1 indicates a completely alpha -helical structure. Calculation of fraction helix is described under "Experimental Procedures." A, alpha -helical content of each polypeptide as determined by CD spectroscopy at 222 nm at 0 °C. Values are an average of three to five individual readings at different concentrations, and error bars represent ±1 standard deviation. B-D, thermal denaturation of the analogues. B, wild-type analogues. C, polypeptides containing L-core. D, polypeptides containing S-core.

An initial inspection of the results (Fig. 3A) for exchanges to wflAFP-6 demonstrated that the effects on helicity for each exchange appeared to be additive. The decreases in helical content between Liver(wt) and [S]Liver (10.3%), and between Liver(wt) and Liver[S] (8.9%), gave a combined decrease of 19.2% that would predict a helical content of 75.3% for [S]Liver[S], which was close to the observed value of 77.9%. However, for wfsAFP-2, replacement of the C terminus alone (Skin[L]) produced ~100% helical content (Fig. 3A), whereas [L]Skin demonstrated ~90% helical content.

Pairwise Comparison of the Effects of the N Terminus, Core Region, and C Terminus on alpha -Helical Content-- The differences in helical content between polypeptides that differed at a single region are summarized in Table I, column 3. Several of the differences were found not to be statistically significant in this comparison; however, in three of these instances, the p values were close to the alpha  value of 0.05 used in the analysis (Table I, column 4, a2, b1, and c2). Overall, the results of the pairwise comparison of the effects of exchanges on helical content were not as consistent as for the activity analysis, because of the aberrant values found for Skin[L] (Table I, column 3). However, if the results were evaluated without Skin[L] (Table I, column 5 in parts A and B), the [L]-Nterm imparted ~8.7% higher helical content than the [S]-Nterm. Conversely, the L-core sequence was ~4.5% less helical than the corresponding S-core region. Although the experimental error would preclude forming conclusions based on the assay of individual polypeptide comparisons, the general trend observed in the pairwise comparison indicated that the [L]-Nterm induced a higher helical content than the [S]-Nterm, whereas the S-core induced a higher helical content than the L-core.

For the C-terminal exchange, the [L]-Cterm always produced higher helical content than [S]-Cterm. Only in the presence of [S]-Nterm and L-core was the increased helical content (Table I, column 3, c2 value) associated with [L]-Cterm found to be statistically insignificant. However, a dependence on the nature of the core sequence for the increased helicity associated with [L]-Cterm was observed, as helical content was ~10% higher when the S-core was present (Table I, column 6). When the L-core was present, the [L]-Nterm demonstrated a greater effect on enhanced helicity in the presence of the [L]-Cterm (8.9 - 6.3% = 2.6%). Conversely, when the S-core was present, the [S]-Nterm provided higher enhancement of helicity in the presence of the [L]-Cterm (16.5% - 20.3% = -3.8%). In both instances, the difference values were based on a single scenario, unlike earlier comparisons where trends could be discerned because of multiple values from independent comparisons. However, these results may indicate that the dependence on the nature of the core region is further enhanced when the core region is associated with its native N terminus. An analysis of the helicity values obtained for the N-terminal exchange demonstrated that the same relationship existed for the N terminus. The effect of higher helical content associated with [L]-Nterm was greater in the presence of L-core, but when either core was present, the increased helical content was higher when each core was associated with its own C terminus (Table I, column 3, A).

Correlation of Activity Levels and Helical Content-- When comparing all analogues studied, activity levels increased as helical content increased (Fig. 4A). However, for all analogues, a rigorous direct correlation between helical content and activity was not observed (Fig. 4A, overall linear regression line). If the L-core and S-core analogues are analyzed separately, the analogues containing L-core demonstrated a very good direct correlation between activity and helical content (R2 = 0.990), whereas the S-core containing analogues still demonstrated a low level of direct correlation. Examination of the residuals for the linear regression for all analogues demonstrated that a reasonably good correlation between activity and helical content existed until the polypeptides achieved a helical content of ~90%, beyond which the correlation became very poor.


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Fig. 4.   A comparison of the observed activity levels and the helical content for each analogue. A, a plot of the correlation between helical content and the activity level, as a percentage of Liver(wt), for each analogue. Error bars in the x and y axes directions are ±1 standard deviation. For Liver(wt), there is no y axis error bar as all activity values were normalized to Liver(wt). The solid black line (regression) is a plot of predicted activities from a linear regression analysis for all analogues. L-core (solid gray line) is a plot of predicted activities from a linear regression analysis for analogues containing L-core, and S-core (broken line) is a plot of predicted activities from analysis of analogues containing S-core. B, plot of the residual values from the linear regression analysis. L-core points are the residuals from analysis of only the L-core-containing analogues, and S-core points are the residuals of the analysis of analogues containing S-core.

Comparison of Observed alpha -Helical Content with Predicted Values Based on a Simple Two-state Helix Prediction Method-- In Table III, the predicted helical contents were derived at by using a simple two-state helix prediction method where each polypeptide component was isolated and assigned a total number of helical residues likely to be found in each region. For wflAFP-6, helix predictions were based on the assumption that each region ([L]-Nterm, L-core, and [L]-Cterm) was 100% helical based on structural data (8, 31). For wfsAFP-2, the assignments were based on current theories of helix capping (see "Discussion" for rationale behind assignment of helical and non-helical residues). In the [S]-Nterm, 3 of 4 residues were assumed to be non-helical (all residues preceding Pro4), the S-core was assumed to be 100% helical, and in [S]-Cterm, 4 of 6 residues were assumed to be non-helical (all residues following and including Gly-36). The predicted helical contents for each polypeptide was then simply arrived at by determining the total number of residues in a helical conformation under the assumption that each region was independent of effects caused by the identity of the other regions. Examination of all polypeptides that contained the S-core demonstrated a remarkably high correlation of the predicted values with the observed values, except for Skin[L], which was underestimated by ~11%. In polypeptides that contained L-core, including Liver(wt), the helical content was consistently overestimated by ~5%.


                              
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Table III
A comparison of predicted alpha -helical content values based on a simple two-state model including helix capping with those observed by CD spectroscopy

Thermal Denaturation of Polypeptides-- The polypeptides were subjected to thermal denaturation from 0 °C to 60, 64, or 65 °C, and their helical contents were assayed by CD spectroscopy at 222 nm (data not shown). The thermal denaturation of each polypeptide was fully reversible, but demonstrated very broad transitions over the temperature ranges used. Because of the broad nature of the unfolding process, standard practices of curve fitting for thermal denaturation data (32, 33) could not be performed on data collected here without producing significantly large values of error (data not shown). Thus, only a qualitative assessment of unfolding is presented by evaluating the helical fraction (fH) of each polypeptide during thermal denaturation.

The two wild-type polypeptides displayed partial cooperativity in helix unfolding as evidenced by "S-shaped" denaturation profiles and a slight degree of thermal stability as temperatures increased (Fig. 3B). At temperatures below ~25 °C, Liver(wt) demonstrated enhanced helical content over Skin(wt). All polypeptides demonstrated some degree of cooperative unfolding except for [S]Liver and [S]Liver[S], which lacked S-shaped unfolding profiles and any indications of thermal stability (Fig. 3C). For [L]Skin, there was only a slight increase in helical content at 0 °C compared with Skin(wt), but an increase in thermal stability was observed (Fig. 3D). For Skin[L], the unfolding process maintained only a slight cooperative nature (Fig. 3D). In [L]Skin[L] (Fig. 3D), thermal stability was enhanced as observed for [L]Skin. Overall, [L]Skin and [L]Skin[L] demonstrated the highest thermal stability of all the polypeptides assayed.

Thr to Ser Mutation in [L]Skin-- To determine the cause of the increased thermal hysteresis observed for [L]Skin, Thr-2 was mutated to Ser, [L(T2S)]Skin (Fig. 5A), which retained the -OH group necessary for the formation of the hydrogen-bonding network in the N terminus that stabilizes the helix structure (8), but removed the gamma -methyl group of Thr that is involved in ice-binding (17, 18, 20, 21). Thus, this mutation was designed to determine whether the increased activity of [L]Skin was the result of an enhanced N-cap function leading to greater helix stability (see "Discussion") or of the introduction of a new, or more efficient, ice-binding surface. The activity of [L(T2S)]Skin was slightly less than Skin(wt) (Fig. 5B); however, no loss of helical content for [L(T2S)]Skin at 0 °C was observed (Fig. 5C). Thus, the improved activity of the [L]Skin mutation was because of the introduction of a more efficient ice-binding surface centered around the gamma -methyl group of Thr-2, and not because of the increased helical content of the entire polypeptide afforded by the exchange of [S]-Nterm by [L]-Nterm.


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Fig. 5.   Increased activity of [L]Skin polypeptide is dependent on presence of gamma -methyl group of Thr-2. A, sequences of the synthetic polypeptides analyzed. All polypeptides were synthesized with free N termini and amidated C termini. The identical residues in the core region between all polypeptides are highlighted in gray. The Thr-2 right-arrow Ser mutation in [L(T2S)]Skin is highlighted in black. B, thermal hysteresis levels of the polypeptides. [L]Skin control is data collected in Fig. 2A and is included for comparison purposes. C, helical fraction of each polypeptide as determined by CD spectroscopy (222 nm) at 0 °C. Values are averages of three to four independent readings, and error bars are ±1 standard deviation.


    DISCUSSION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Taking into account the results of individual exchanges, the pairwise comparison, and earlier studies,2 we conclude that the ~50% difference in antifreeze activity between wflAFP-6 and wfsAFP-2 is derived from (i) average contributions of ~20% by both the N (DTASDA versus MDAP) and C termini (AR versus KAGAAR), and (ii) a 10% contribution by the core region (complete IBM (LTAAN) versus incomplete IBM (ATAAA)). Furthermore, the magnitude of change in antifreeze activity generated by the exchange of a wfsAFP-2 component with a wflAFP-6 component was dependent on the characteristics of the other polypeptide regions. The region that imparted the greatest influence on activity between wfsAFP-2 and wflAFP-6 was the N terminus, because of its own ability to modulate activity levels and its influence on the activity of other regions of the polypeptide. The termini of wflAFP-6 demonstrated a greater ability to impart both higher helical character and thermal stability as compared with the wfsAFP-2 termini. However, the wflAFP-6 core region exhibited lower helix propensity than the wfsAFP-2 core region. Thus, the activity level of each region is likely related to a complex interplay between its own inherent ice-binding ability, helix propensity, and the helix propensity imparted upon the entire polypeptide by each region.

The thermal hysteresis levels associated with type I AFPs have been shown to be positively correlated with helical content (34), which is likely the result of the ability of ice-binding residues to adopt the proper configuration for ice recognition. This positive correlation of activity with helical content was confirmed with the analogues studied here (Fig. 4). However, the results clearly demonstrated that other factors as well as helical content affect activity levels, especially after relatively high helical content (>~90%) is achieved, an example of which was demonstrated by the [L(T2S)]Skin mutation. Furthermore, a more direct correlation was observed for analogues containing L-core than for S-core, indicating that the activity of analogues containing L-core were more sensitive to the helical content.

From current theories of helix capping, it can be predicted that Gly-36 of wfsAFP-2 occupies the C' position in a C-cap, or at least acts as a helix terminator, and Pro-4 is constrained to occupy the N1 position of the N-cap under the conventional notation for residues at helix termini (35). If all intervening residues adopt alpha -helical (phi , psi ) angles, the predicted helical content of Skin(wt) would be ~80%, which is very close to the observed value of ~82% (see Fig. 3A). Thus, from this analysis, the helix propensity of the S-core is equivalent to, or more likely, greater than (see below) the helix propensity of the L-core (at 0 °C), even though the CD measurements consistently demonstrated a lower overall helical content at 0 °C for wfsAFP-2. The nearly identical helical content of [S]Liver[S] to Skin(wt) at 0 °C (~78% versus ~82%) could be interpreted in the same manner as for Skin(wt). However, the lack of thermal stability of [S]Liver[S] compared with Skin(wt) (see Fig. 3C) would suggest that the L-core possesses a lower helical propensity than the S-core, which would be expected because of the higher Ala content in the S-core (36). Furthermore, the L-core consistently demonstrated a lower helical content than S-core (Table I, column 2, B). The assessment of a slightly lower than 100% helical propensity for L-core led to an overestimation of the helical content for polypeptides containing L-core in the simple two-state helix prediction model (see Table III). The analysis presented in Table III was not an attempt to fully describe the structural characteristics of type I AFPs, but was used merely to illustrate that, in direct comparison, L-core was in fact not 100% helical whereas S-core maintains high helical content under several differing contexts. Thus, the S-core contributed more overall helical character than L-core when present in type I AFPs. Furthermore, the lower helix propensity of L-core compared with S-core manifested itself in the correlation between helical content and activity (Fig. 4), where the activity levels were more directly dependent on helical content for analogues containing L-core than for those containing S-core. Thus, although L-core improved the activity compared with S-core, the presence of complete IBMs lowered the helical propensity within the core, which led to the observed higher correlation between activity and helical content for L-core-containing polypeptides.

Helix capping refers to patterns of hydrogen bonding and hydrophobic interactions present at the termini of alpha -helices that satisfy residues that do not possess main-chain amide hydrogen to carbonyl oxygen hydrogen bonding partners of the form i right-arrow i + 4 that are found in the core of the helix (35). As evident from the crystal structure, such helix termini capping networks exist in wflAFP-6 (8). Furthermore, helix-capping ability would lead to a lower nucleation barrier for helix formation and, thus, greater thermal stability and helical content for the entire helix, because it has been suggested that helix caps can exert a significant effect on helix nucleation (37). Thus, inherent in a higher propensity for helix cap formation is a greater ability to impart helical character to the entire polypeptide. The ability of [L]-Nterm to impart higher thermal stability and its consistent demonstration of the ability to impart higher helical content to the entire polypeptide at 0 °C may indicate a greater N-capping propensity for [L]-Nterm compared with [S]-Nterm. In native winter flounder AFPs, the higher helix-inducing ability of the [L]-termini as compared with the corresponding [S]-termini may be necessitated by the lower helix propensity of the L-core caused by the presence of the more active complete IBMs. Thus, when L-core replaced S-core in [S]Liver[S], only a ~3% increase in activity was noted (see Table I) because the [S]-termini were not able to promote a high enough helical content within the core region to produce the full antifreeze activity of L-core. Conversely, nearly the full magnitude of the effect on activity for the core exchange was observed in [L]Skin[L], because all components in this polypeptide were able to produce maximal helical content.

In wfsAFP-2, Lys-6, which is normally found i + 4 to Asp-2, was not transferred along with [S]-Nterm in the various exchanges. The Asp-2/Lys-6 pair (see Fig. 1, D2-K6) may be necessary to form a salt bridge to stabilize the helix by forming an N-cap. Furthermore, the C terminus of wfsAFP-2 may be involved in a complex C-cap structure, because C-capping residues usually reside outside the helix proper and often require a Gly residue at C' to allow for positive (phi , psi ) angles (35). Although the lower capping ability of [S]-Nterm may suggest that the Asp-2/Lys-6 salt bridge is necessary in wfsAFP-2, the improved thermal stability of [L]Skin over Skin(wt) would suggest that [L]-Nterm still possessed a superior ability to impart higher helix propensity to the entire polypeptide. Furthermore, the inherent thermal stability of the S-core suggests that the helix-nucleating capabilities of the termini are not as critical for S-core. The putative Asp-2/Lys-6 salt bridge may also explain the seemingly aberrant results observed for Skin[L] in that some form of interaction between regions caused the three residues preceding Pro-4 to adopt a helical conformation. Further work is necessary to investigate the validity of the proposed Asp-2/Lys-6 salt bridge.

The "long range" dependence of the increased activity associated with each [L]-termini on the identities of the opposing termini was likely related to the relative helix propensity of the remainder of the polypeptide. Thus, the order of the activity dependence (N terminus > C terminus > core) was a reflection of the importance of each region on the overall helix propensity. The placement of the core last in the order does not imply that the helix propensity of the core is inconsequential to activity. The low level of influence was observed because both L-core and S-core were highly helical, and exchanges between the two likely did not significantly influence the character at the termini or significantly change the nature of the hydrophobic binding face. However, relatively distant termini likely affected the activity through their ability to induce helical content to the overall polypeptide through helix capping, thereby enhancing the ice-binding sites in other portions of the polypeptide.

In wflAFP-6, the first 11-residue motif occurs in the N terminus. A study of a minimized peptide consisting of the N and C termini of wflAFP-6 (38) and mutagenesis studies performed on the first and last Thr residues of wflAFP-6 (21) have suggested a role for the N terminus in activity. The Thr right-arrow Ser mutation in [L(T2S)]Skin clearly demonstrated that Thr-2 is involved in antifreeze activity. However, in a previous study, it was found that the first four residues of wflAFP-6 could be deleted with no effect on activity (27). It should be noted that there are no reports of a single mutation (T2S) in wflAFP-6 (7), and further work is necessary to identify the cause of these opposing results.

The magnitude of the detrimental effect of replacing [L]-Nterm with [S]-Nterm was greater than the magnitude of the enhancement for the opposite exchange. This may reflect the fact that, in [S]Liver, the loss of activity was the result of a combination of lower helical content afforded by [S]-Nterm, which affected the ice-binding sites of the remainder of the polypeptide, and more importantly, the loss of a highly active ice-binding site within [L]-Nterm itself. In contrast in the opposite exchange, Skin(wt) to [L]Skin, the increased activity was only the result of the introduction of a more efficient ice binding site, and the improved helicity only minimally affected the remainder of the ice binding sites, because of the inherently high helical content associated with S-core. At the C terminus, the low level of evolutionary conservation (7) indicates that this region is less likely to be critical for biological activity. The increased activity with [L]-Cterm over [S]-Cterm may be caused in part by the presence of a more efficient capping structure, which resulted in a lower entropic cost to ice binding, as no sacrifice of conformational entropy at the C terminus was necessary upon ice binding. Nevertheless, the results also suggest that [L]-Cterm may have an enhanced ice binding ability over [S]-Cterm, in a similar manner as described for the N termini.

The data obtained in this study have demonstrated that there is a complex relationship between the helical propensities of the different regions of type I AFPs (N terminus, core, and C terminus) and the level of antifreeze activity. Thus, the conclusions presented here should be used as a first step in more in-depth studies of the determinants of antifreeze activity that reside in the N and C termini of other type I AFPs.

    ACKNOWLEDGEMENTS

We thank Dr. Frank D. Sönnichsen for critical review of an original draft of the manuscript, Dr. Nam-Chiang Wang for peptide synthesis, Rey Interior for amino acid analysis, Dr. Avijit Chakrabartty for assistance with CD spectroscopy, Dr. Daniel S. C. Yang for helpful discussions, and Cora Young for assistance with preparation of the manuscript.

    FOOTNOTES

* This work was supported in part by grants from the Canadian Institutes of Health Research (formerly the Medical Research Council, Canada) (to C. L. H.).The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

Recipient of an Ontario graduate scholarship.

Dagger Dagger To whom correspondence should be addressed: Dept. of Biological Sciences, National University of Singapore, Singapore 119260, Singapore. Tel.: 65-6874-2692; Fax: 65-6779-2486; E-mail: dbshead@nus.edu.sg.

Published, JBC Papers in Press, January 13, 2003, DOI 10.1074/jbc.M300081200

2 Q. Lin, W. Low, and C. L. Hew, manuscript in preparation.

    ABBREVIATIONS

The abbreviations used are: AFP, antifreeze protein/polypeptide; AFGP, antifreeze glycoprotein; wflAFP, winter flounder liver-type AFP; wfsAFP, winter flounder skin-type AFP; HPLC, high performance liquid chromatography; IBM, ice-binding motif; CD, circular dichroism; wt, wild-type; [L]-Nterm, liver-type N terminus; [L]-Cterm, liver-type C terminus; L-core, liver-type core; [S]-Nterm, skin-type N terminus; [S]-Cterm, skin-type C terminus; S-core, skin-type core; Fmoc, N-(9-fluorenyl)methoxycarbonyl.

    REFERENCES
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
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