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首页> 外文期刊>The Journal of Physiology >Relationship between anion binding and anion permeability revealed by mutagenesis within the cystic fibrosis transmembrane conductance regulator chloride channel pore.
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Relationship between anion binding and anion permeability revealed by mutagenesis within the cystic fibrosis transmembrane conductance regulator chloride channel pore.

机译:囊性纤维化跨膜电导调节剂氯离子通道孔中的诱变揭示了阴离子结合与阴离子渗透性之间的关系。

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1. Anion binding within the pores of wild-type and mutant cystic fibrosis transmembrane conductance regulator (CFTR) Cl- channels, expressed in two different mammalian cell lines, was assayed using patch clamp recording. Specifically, experiments measured both the conductance of different anions and the ability of other permeant anions to block Cl- permeation through the pore. 2. Under symmetrical ionic conditions, wild-type CFTR channels showed the conductance sequence Cl- > NO3- > Br- > or = formate > F- > SCN- congruent to ClO4-. 3. High SCN- conductance was not observed, nor was there an anomalous mole fraction effect of SCN- on conductance under the conditions used. Iodide currents could not be measured under symmetrical ionic conditions, but under bi-ionic conditions I- conductance appeared low. 4. Chloride currents through CFTR channels were blocked by low concentrations (10 mM) of SCN-, I- and ClO4-, implying relatively tight binding of these anions within the pore. 5. Two mutations in CFTR which alter the anion permeability sequence, F337S and T338A, also altered the anion conductance sequence. Furthermore, block by SCN-, I- and ClO4- were weakened in both mutants. Both these effects are consistent with altered anion binding within the pore. 6. The effects of mutations on anion permeability and relative anion conductance suggested that, for most anions, increased permeability was associated with increased conductance. This indicates that the CFTR channel pore does not achieve its anion selectivity by selective anion binding within the mutated region. Instead, it is suggested that entry of anions into the region around F337 and T338 facilitates their passage through the pore. In wild-type CFTR channels, anion entry into this crucial pore region is probably dominated by anion hydration energies.
机译:1.使用膜片钳记录法测定了在两种不同哺乳动物细胞系中表达的野生型和突变型囊性纤维化跨膜电导调节剂(CFTR)Cl-通道内的阴离子结合。具体而言,实验测量了不同阴离子的电导率以及其他渗透阴离子阻止Cl-渗透通过孔的能力。 2.在对称离子条件下,野生型CFTR通道显示与ClO4-一致的电导序列Cl-> NO3-> Br->或=甲酸> F-> SCN-。 3.在所使用的条件下,未观察到高的SCN-电导,也没有异常的SCN-摩尔分数对电导的影响。在对称离子条件下无法测量碘化物电流,但在双离子条件下,I导率显得较低。 4.通过CFTR通道的氯离子电流被低浓度(10 mM)的SCN-,I-和ClO4-阻断,这意味着这些阴离子在孔内的结合相对紧密。 5. CFTR中的两个改变阴离子渗透性的序列F337S和T338A也改变了阴离子电导序列。此外,在两个突变体中,SCN-,I-和ClO4-的阻断作用均减弱。这两种作用与孔内阴离子结合的改变是一致的。 6.突变对阴离子渗透率和相对阴离子电导的影响表明,对于大多数阴离子而言,渗透率的增加与电导率的增加有关。这表明CFTR通道孔不能通过突变区域内的选择性阴离子结合而达到其阴离子选择性。相反,建议阴离子进入F337和T338周围区域有助于它们穿过孔。在野生型CFTR通道中,阴离子进入这个关键的孔区域可能是由阴离子水合能量所主导。

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