通过暴露于氨基乙酰丙酸刺激培养的哺乳动物上皮细胞中的四吡咯合成。
Stimulation of tetrapyrrole synthesis in mammalian epithelial cells in culture by exposure to aminolaevulinic acid.
作者信息
Washbrook R, Fukuda H, Battle A, Riley P
机构信息
Department of Molecular Pathology, UCL Medical School, London, UK.
出版信息
Br J Cancer. 1997;75(3):381-7. doi: 10.1038/bjc.1997.62.
Tetrapyrrole synthesis in CNCM-1221 cells exposed to 0.6 mM aminolaevulinic acid (ALA) was found to be approximately linear over a 6-h period of incubation. The rate was not significantly affected by cell density over a range of 0.015 to 0.15 x 10(6) cells cm(-2) (final cell density). Tetrapyrrole synthesis was not affected by GABA or glutamic acid in concentrations up to 6 mM and 2.72 mM respectively, suggesting that these amino acids, which are similar in structure to ALA, do not competitively inhibit the ALA uptake pathway in these cells. Pre-exposure to haem arginate (up to 100 microM) was inhibitory, presumably by suppression (through the inhibition of ALA synthase) of an endogenous component of the response. The ALA-stimulated response was not modified by co-exposure to AIA (up to 100 mg ml(-1)). Despite significant reduction of protein synthesis, the porphyrinogenic response of cells exposed to ALA was unaffected by cycloheximide (10 microg ml(-1)) or actinomycin D (10 microg ml(-1)) even when cells were preincubated with these agents for 3 h before ALA exposure. Fetal bovine serum (10%) inhibited tetrapyrrole synthesis by 30% but increased the rate of porphyrin export by cells by a factor of 1.5. The uptake of [14C]ALA was shown to be strongly influenced by the density of the cultures. In dense cultures (final cell density of approximately 0.15 x 10(6) cells cm(-2)), the ALA uptake rate was less than 0.8 compared with a maximum rate of 4.2 fmol per cell h(-1) at a cell density of 0.02 x 10(6) cells cm(-2). Since tetrapyrrole synthesis is less affected than ALA uptake by cell density, the resultant discrepancy in ALA incorporation occurring in dense cultures implies that endogenous ALA synthesis is induced in these cells. ALA uptake was not affected by cycloheximide or actinomycin D in serum-free conditions. However, fetal bovine serum decreased external ALA uptake by about 50%. This effect was abrogated by preincubation with cycloheximide.
在暴露于0.6 mM氨基乙酰丙酸(ALA)的CNCM - 1221细胞中,四吡咯合成在6小时的孵育期内大致呈线性。在0.015至0.15×10⁶个细胞/cm²(最终细胞密度)的范围内,细胞密度对速率没有显著影响。四吡咯合成不受分别高达6 mM和2.72 mM的GABA或谷氨酸的影响,这表明这些结构与ALA相似的氨基酸不会竞争性抑制这些细胞中的ALA摄取途径。预先暴露于血红素精氨酸(高达100 μM)具有抑制作用,推测是通过抑制(通过抑制ALA合酶)反应的内源性成分。同时暴露于AIA(高达100 mg/ml)不会改变ALA刺激的反应。尽管蛋白质合成显著减少,但暴露于ALA的细胞的卟啉生成反应不受放线菌酮(10 μg/ml)或放线菌素D(10 μg/ml)的影响,即使在ALA暴露前将细胞与这些试剂预孵育3小时也是如此。胎牛血清(10%)使四吡咯合成减少30%,但使细胞的卟啉输出速率提高了1.5倍。[¹⁴C]ALA的摄取显示受培养物密度的强烈影响。在高密度培养物(最终细胞密度约为0.15×10⁶个细胞/cm²)中,ALA摄取速率小于0.8,而在细胞密度为0.02×10⁶个细胞/cm²时,最大摄取速率为4.2 fmol/细胞·h⁻¹。由于细胞密度对四吡咯合成的影响小于对ALA摄取的影响,在高密度培养物中发生的ALA掺入的差异意味着这些细胞中诱导了内源性ALA合成。在无血清条件下,ALA摄取不受放线菌酮或放线菌素D的影响。然而,胎牛血清使外部ALA摄取减少约50%。用放线菌酮预孵育可消除这种作用。
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