Yuan Tao, Fournier Anick R, Proudlock Raymond, Marshall William D
Department of Food Science and Agricultural Chemistry, MacDonald Campus of McGill University, 21111 Lakeshore Road, Ste-Anne-de-Bellevue, Quebec, Canada.
Environ Sci Technol. 2007 Mar 15;41(6):1983-8. doi: 10.1021/es062194+.
A continuous hydrogenation device was evaluated for the detoxification of selected tri-, tetra-, or pentacyclic polyaromatic hydrocarbon (PAH) compounds {anthracene, phenanthrene, chrysene, and benzo[a]pyrene (B[a]P)} by hydrogenation. A substrate stream in hexane, 0.05-1.0% (w/v), was mixed with hydrogen-carbon dioxide (H2-CO2, 5-30% v/v) and delivered to a heated reactor column (25 cm x 1 cm) containing palladium supported on gamma alumina (Pd0/gamma-Al2O3) that was terminated with a capillary restrictor. The flow rate from the reactor, approximately 800 mL min(-1) decompressed gas, corresponded to 4 mL min(-1) fluid under the operating conditions of the trials. Reaction products were recovered by passing the reactor effluent through hexane. At 90 degrees C, the anthracene or phenanthrene substrate was hydrogenated only partially to octahydro and dodecahydro species and contained only a minor quantity of totally hydrogenated products. For substrates with increasing numbers of fused aromatic rings, the hydrogenation efficiency was decreased further. However, at an increasing temperature (90-150 degrees C) and increasing mobile phase flow rate (20.68 MPa corresponding to 2100 mL min(-1) decompressed gas), B[a]P and chrysene were hydrogenated, virtuallytotally, to their corresponding perhydro analogues (eicosahydrobenzo[a]pyrenes and octadecahydrochrysenes), respectively. That this approach might be useful for decontaminating soil extracts was supported by companion in vitro trials in which the substrate and products were assayed for mutagenic activity with five bacterial strains that are auxotrophic for histidine (Salmonella typhimurium TA98, TA100, TA1535, and TA1537) or tryptophan (Escherichia coliWP2 uvrA), using the bacterial reverse mutation assay (modified Ames test). Generally, substantial increases in revertant colony counts were not observed with any of the strains following exposure to the hydrogenation products in the absence or presence of the 10 or 30% S9 mix, which is consistent with the loss of mutagenic activity from these hydrogenation products.
对一种连续氢化装置进行了评估,该装置用于通过氢化作用对选定的三环、四环或五环多环芳烃(PAH)化合物{蒽、菲、芘和苯并[a]芘(B[a]P)}进行解毒。将己烷中的底物流(0.05 - 1.0%,w/v)与氢气 - 二氧化碳(H₂ - CO₂,5 - 30% v/v)混合,然后输送到一个装有负载在γ - 氧化铝上的钯(Pd⁰/γ - Al₂O₃)的加热反应器柱(25 cm×1 cm)中,该反应器柱末端装有毛细管限流器。反应器的流速约为800 mL min⁻¹减压气体,在试验的操作条件下相当于4 mL min⁻¹流体。通过使反应器流出物通过己烷来回收反应产物。在90℃时,蒽或菲底物仅部分氢化为八氢和十二氢物种,并且仅含有少量完全氢化的产物。对于稠合芳环数量增加的底物,氢化效率进一步降低。然而,在温度升高(90 - 150℃)和流动相流速增加(20.68 MPa相当于2100 mL min⁻¹减压气体)的情况下,B[a]P和芘分别几乎完全氢化为它们相应的全氢类似物(二十氢苯并[a]芘和十八氢芘)。该方法可能对土壤提取物的去污有用,这一点得到了配套体外试验的支持,在这些试验中,使用细菌回复突变试验(改良的艾姆斯试验),用五种对组氨酸(鼠伤寒沙门氏菌TA98、TA100、TA1535和TA1537)或色氨酸(大肠杆菌WP2 uvrA)营养缺陷的细菌菌株,对底物和产物的诱变活性进行了测定。一般来说,在不存在或存在10%或30% S9混合物的情况下,暴露于氢化产物后,任何菌株的回复菌落数均未观察到显著增加,这与这些氢化产物诱变活性的丧失一致。
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