Winkler E, Klingenberg M
Institute of Physical Biochemistry, University of Munich, Federal Republic of Germany.
Eur J Biochem. 1992 Jan 15;203(1-2):295-304. doi: 10.1111/j.1432-1033.1992.tb19859.x.
The nucleotide binding center of the uncoupling protein from brown adipose tissue (UCP) was probed by photoaffinity labeling with 8-azido-ATP. The isolated dimeric UCP in non-ionic detergent was used. 8-azido-ATP binds to UCP with a Kd = 3 microM, i.e. with an only threefold lower affinity than ATP and a maximum number of binding sites of about 12 mumol/g protein corresponding to about 1 mol/mol dimer UCP. UCP is rapidly degraded by ultraviolet radiation, and therefore only near ultraviolet and visible light can be used for photoaffinity labeling. The total covalent incorporation is shown to be dependent on the concentration of azido-ATP and on competing phospholipids. The specific, i.e. ATP-sensitive incorporation only to the binding site depends on the presence of cysteine. With CNBr cleavage the 8-azido-[gamma-32P]ATP insertion within the primary structure was located by identifying ATP-sensitive labeled peptides in SDS/PAGE. A major specific 8-azido-ATP incorporation was found by autoradiography in the smallest CNBr fragments. Identification of the radioactive peptides was difficult since 8-azido-ATP insertion causes a distinct shift in the gels from the stained peptides. Identification was possible by specific disulfide formation at the C-terminal within the UCP dimer which only removed the CB7 (CB, CNBr fragment) portion of the low-molecular-mass peptides but did not move the radioactive band. This excludes the C-terminal CB7 and identifies the labeled peptide as CB6. Also, limited tryptic cleavage of intact UCP at Lys293 did not remove the radioactivity. Cleavage of tryptophanes support localization of 8-azido-ATP between residues 173-280 which includes CB6. Solid-phase sequencing of the labeled CB6 both after serine lactone and carboxyl coupling suggest incorporation into Thr260. These results indicate that the adenine-binding site is within the third domain of the tripartite UCP structure at a putative hydrophilic channel which can be assessed both from the cytosol and matrix of mitochondria.
利用8-叠氮基-ATP进行光亲和标记,对棕色脂肪组织解偶联蛋白(UCP)的核苷酸结合中心进行了研究。使用的是在非离子去污剂中分离得到的二聚体UCP。8-叠氮基-ATP以Kd = 3 microM的亲和力与UCP结合,即其亲和力仅比ATP低三倍,最大结合位点数约为12 μmol/g蛋白,相当于约1 mol/mol二聚体UCP。UCP会被紫外线迅速降解,因此光亲和标记只能使用近紫外光和可见光。总的共价掺入显示取决于叠氮基-ATP的浓度以及竞争性磷脂。特异性的,即仅对结合位点的ATP敏感掺入取决于半胱氨酸的存在。通过CNBr裂解,通过在SDS/PAGE中鉴定ATP敏感的标记肽段,确定了8-叠氮基-[γ-32P]ATP在一级结构中的插入位置。通过放射自显影在最小的CNBr片段中发现了主要的特异性8-叠氮基-ATP掺入。由于8-叠氮基-ATP的插入导致凝胶中染色肽段明显移位,因此难以鉴定放射性肽段。通过在UCP二聚体的C端形成特异性二硫键,使得鉴定成为可能,该二硫键仅去除了低分子量肽段的CB7(CB,CNBr片段)部分,但没有移动放射性条带。这排除了C端的CB7,并将标记肽段鉴定为CB6。此外,在Lys293处对完整UCP进行有限的胰蛋白酶裂解并未去除放射性。色氨酸的裂解支持8-叠氮基-ATP定位在包括CB6的173 - 2
