Putilina Tatiana, Skouri-Panet Fériel, Prat Karine, Lubsen Nicolette H, Tardieu Annette
Laboratoire de Minéralogie-Cristallographie, CNRS and P6-P7 Universities, Case 115, 4 Place Jussieu, F75252 Paris Cedex 05, France.
J Biol Chem. 2003 Apr 18;278(16):13747-56. doi: 10.1074/jbc.M208157200. Epub 2003 Jan 31.
The chaperone activity of native alpha-crystallins toward beta(LOW)- and various gamma-crystallins at the onset of their denaturation, 60 and 66 degrees C, respectively, was studied at high and low crystallin concentrations using small angle x-ray scattering (SAXS) and fluorescence energy transfer (FRET). The crystallins were from calf lenses except for one recombinant human gamma S. SAXS data demonstrated an irreversible doubling in molecular weight and a corresponding increase in size of alpha-crystallins at temperatures above 60 degrees C. Further increase is observed at 66 degrees C. More subtle conformational changes accompanied the increase in size as shown by changes in environments around tryptophan and cysteine residues. These alpha-crystallin temperature-induced modifications were found necessary to allow for the association with beta(LOW)- and gamma-crystallins to occur. FRET experiments using IAEDANS (iodoacetylaminoethylaminonaphthalene sulfonic acid)- and IAF (iodoacetamidofluorescein)-labeled subunits showed that the heat-modified alpha-crystallins retained their ability to exchange subunits and that, at 37 degrees C, the rate of exchange was increased depending upon the temperature of incubation, 60 or 66 degrees C. Association with beta(LOW)- (60 degrees C) or various gamma-crystallins (66 degrees C) resulted at 37 degrees C in decreased subunit exchange in proportion to bound ligands. Therefore, beta(LOW)- and gamma-crystallins were compared for their capacity to associate with alpha-crystallins and inhibit subunit exchange. Quite unexpectedly for a highly conserved protein family, differences were observed between the individual gamma-crystallin family members. The strongest effect was observed for gamma S, followed by h gamma Srec, gamma E, gamma A-F, gamma D, gamma B. Moreover, fluorescence properties of alpha-crystallins in the presence of bound beta(LOW)-and gamma-crystallins indicated that the formation of beta(LOW)/alpha- or gamma/alpha-crystallin complexes involved various binding sites. The changes in subunit exchange associated with the chaperone properties of alpha-crystallins toward the other lens crystallins demonstrate the dynamic character of the heat-activated alpha-crystallin structure.
利用小角X射线散射(SAXS)和荧光能量转移(FRET)技术,在高、低晶状体蛋白浓度下,研究了天然α-晶状体蛋白在β(LOW)-晶状体蛋白和各种γ-晶状体蛋白变性起始温度(分别为60℃和66℃)时的伴侣活性。除一种重组人γS外,其余晶状体蛋白均来自小牛晶状体。SAXS数据表明,在60℃以上的温度下,α-晶状体蛋白的分子量不可逆地翻倍,且尺寸相应增大。在66℃时观察到进一步增大。色氨酸和半胱氨酸残基周围环境的变化表明,随着尺寸增大,构象变化更为细微。发现这些α-晶状体蛋白温度诱导的修饰是其与β(LOW)-晶状体蛋白和γ-晶状体蛋白发生缔合所必需的。使用IAEDANS(碘乙酰氨基乙基氨基萘磺酸)和IAF(碘乙酰氨基荧光素)标记亚基的FRET实验表明,热修饰的α-晶状体蛋白保留了亚基交换能力,并且在37℃时,交换速率根据孵育温度(60℃或66℃)而增加。与β(LOW)-(60℃)或各种γ-晶状体蛋白(66℃)缔合后,在37℃时亚基交换速率与结合配体成比例降低。因此,比较了β(LOW)-和γ-晶状体蛋白与α-晶状体蛋白缔合并抑制亚基交换的能力。对于一个高度保守的蛋白质家族而言,相当出乎意料的是,在各个γ-晶状体蛋白家族成员之间观察到了差异。γS的作用最强,其次是hγSrec、γE、γA-F、γD、γB。此外,在结合β(LOW)-和γ-晶状体蛋白的情况下,α-晶状体蛋白的荧光特性表明,β(LOW)/α-或γ/α-晶状体蛋白复合物的形成涉及多个结合位点。与α-晶状体蛋白对其他晶状体蛋白的伴侣特性相关的亚基交换变化证明了热激活的α-晶状体蛋白结构的动态特性。
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