Functional characterization and expression of folate receptor-α in T47D human breast cancer cells

Jwala Renukuntla, Sujay J. Shah, S. H. Boddu, A. Vadlapudi, R. Vadlapatla, D. Pal, A. Mitra
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引用次数: 9

Abstract

Purpose: The objective of this study was to investigate the functional and molecular expression of a carrier mediated system responsible for folate uptake in breast cancer (BC) (T47D) cells and to delineate the mechanism of intracellular regulation of this transport system. Materials and Methods: [ 3 H]-folic acid uptake was studied in T47D cells with respect to time, pH, temperature, sodium and chloride ion dependency. Inhibition studies were conducted in the presence structural analogs, vitamins, metabolic and membrane transport inhibitors. [ 3 H]-folic acid uptake was also determined with varying concentrations of cold folic acid. Uptake kinetics was studied in the presence of various modulators of intracellular regulatory pathways; calcium-calmodulin, protein kinases A and C (PKA and PKC) and protein tyrosine kinase (PTK). Molecular evidence was studied by qualitative and quantitative polymerase chain reaction (PCR) and Western blot analysis. Results: Linear increase in [ 3 H]-folic acid uptake was observed over 30 min. The process followed saturation kinetics with an apparent K m of 11.05 nM, V max of 1.54 FNx01 10−8 μmoles/min/mg proteins and K d of 9.71 FNx01 10−6 /min for folic acid. Uptake process was found to be dependent on pH, sodium ions, chloride ions, temperature and energy. Uptake was inhibited in the presence of structural analogs (cold folic acid, methyltetrahydro folate and methotrexate), but structurally unrelated vitamins did not show any effect. Membrane transport inhibitors such as SITC, DIDS, probenecid and endocytic inhibitor colchicine significantly inhibited the [ 3 H]-folic acid uptake process. PKA, PTK and Ca 2+ /calmodulin pathways positively regulate the uptake process. Reverse transcriptase polymerase chain reaction (RT PCR) analysis had shown mRNA expression of folate receptor (FR)-α at 407 bp. Quantitative polymerase chain reaction analysis showed significantly higher FR-α mRNA levels in T47D cells compared to MCF-7 cells and Western blot analysis confirmed the FR-α protein expression at 37 kDa. Conclusions: This work demonstrated the functional characterization and molecular presence of FR-α in the T47D cell line. The high expression of FRs in T47D human breast carcinoma cells supports their validity as molecular therapeutic targets in BC.
叶酸受体-α在T47D人乳腺癌细胞中的功能表征及表达
目的:本研究的目的是研究乳腺癌(BC) (T47D)细胞中负责叶酸摄取的载体介导系统的功能和分子表达,并描述该运输系统的细胞内调节机制。材料与方法:研究T47D细胞对[3h]-叶酸的摄取对时间、pH、温度、钠离子和氯离子的依赖性。在结构类似物、维生素、代谢和膜运输抑制剂的存在下进行了抑制研究。[3h]-叶酸摄取也测定了不同浓度的冷叶酸。在细胞内调节途径的各种调节剂存在的情况下,研究了摄取动力学;钙钙调素,蛋白激酶A和C (PKA和PKC)和蛋白酪氨酸激酶(PTK)。采用定性和定量的聚合酶链反应(PCR)和Western blot方法研究分子证据。结果:在30 min内,[3 H]-叶酸摄取量呈线性增加,符合饱和动力学,叶酸的表观K m为11.05 nM, V max为1.54 FNx01 10−8 μmol /min/mg蛋白,K d为9.71 FNx01 10−6 /min。发现吸收过程依赖于pH、钠离子、氯离子、温度和能量。在结构类似物(冷叶酸、甲基四氢叶酸和甲氨蝶呤)的存在下,摄取受到抑制,但结构无关的维生素没有表现出任何影响。膜转运抑制剂如SITC、DIDS、probenecid和内吞抑制剂秋水仙碱显著抑制[3 H]-叶酸摄取过程。PKA, PTK和ca2 + /钙调素途径正调控摄取过程。逆转录聚合酶链反应(RT - PCR)显示叶酸受体(FR)-α mRNA在407 bp处表达。定量聚合酶链反应分析显示,T47D细胞中FR-α mRNA水平明显高于MCF-7细胞,Western blot分析证实FR-α蛋白在37 kDa处表达。结论:本工作证实了FR-α在T47D细胞系中的功能表征和分子存在。FRs在T47D人乳腺癌细胞中的高表达支持了其作为乳腺癌分子治疗靶点的有效性。
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