Lobeck K, Drevet P, Léonetti M, Fromen-Romano C, Ducancel F, Lajeunesse E, Lemaire C, Ménez A
CEA, Départment d'Ingénierie et d'Etudes des Protéines, Centre d'Etudes de Saclay, Gif-sur-Yvette, France.
Infect Immun. 1998 Feb;66(2):418-23. doi: 10.1128/IAI.66.2.418-423.1998.
Two recombinant fragments of diphtheria toxin (DT) were fused to an engineered tandem repeat of the immunoglobulin (Ig) binding domain of protein A, called ZZ. These fragments are (i) the receptor binding domain (DTR), which comprises amino acids 382 to 535 of DT, and (ii) a linear peptide (DT(168-220)) which comprises residues 168 to 220 of the loop between fragment A and fragment B of DT. The fusion proteins were produced in Escherichia coli and purified by affinity chromatography. In vitro experiments showed that the DTR domain is responsible for the capacity of ZZ-DTR to bind to Vero cells and is capable of inhibiting the cytotoxicity of DT for these cells. These findings suggest that DTR binds to the cell surface receptors of DT and hence adopts a conformation that is similar to that of the receptor binding domain of DT. We compared the capacities of ZZ-DTR, ZZ-DT(168-220), and a chemically detoxified form of DT currently used for vaccination to elicit antibodies in rabbits. The toxoid was more immunogenic than ZZ-DT(168-220), which in turn was more immunogenic than ZZ-DTR. However, ZZ-DT(168-220) antiserum was poorly efficient at neutralizing DT cytotoxicity on Vero cells, whereas ZZ-DTR antiserum was only 15-fold less potent than anti-DT antisera.
将白喉毒素(DT)的两个重组片段与蛋白A免疫球蛋白(Ig)结合域的工程化串联重复序列(称为ZZ)融合。这些片段为:(i)受体结合域(DTR),其包含DT的第382至535位氨基酸;(ii)线性肽(DT(168 - 220)),其包含DT片段A和片段B之间环的第168至220位残基。融合蛋白在大肠杆菌中产生,并通过亲和层析纯化。体外实验表明,DTR结构域负责ZZ - DTR与Vero细胞结合的能力,并能够抑制DT对这些细胞的细胞毒性。这些发现表明,DTR与DT的细胞表面受体结合,因此采用了与DT受体结合域相似的构象。我们比较了ZZ - DTR、ZZ - DT(168 - 220)以及目前用于疫苗接种的化学解毒形式的DT在兔体内引发抗体的能力。类毒素比ZZ - DT(168 - 220)更具免疫原性,而ZZ - DT(168 - 220)又比ZZ - DTR更具免疫原性。然而,ZZ - DT(168 - 220)抗血清在中和Vero细胞上的DT细胞毒性方面效率低下,而ZZ - DTR抗血清的效力仅比抗DT抗血清低15倍。