Clay Emily M, Shi Xiaohai, Kolar Elizabeth A, Mody Mayur, Locke John E, Watkins Paul A
bioRxiv. 2025 Jul 3:2025.07.02.662811. doi: 10.1101/2025.07.02.662811.
Brain tumors, in particular glioblastoma multiforme (GBM), are among the most aggressive and difficult to treat human neoplasms. Even with combined surgery, radiation and chemotherapy, the 5-year survival rate for GBM is only ∼7%. Thus, new treatment approaches are needed. We previously found that the fatty acid metabolism enzyme "very long-chain acyl-CoA synthetase 3" (ACSVL3) is overproduced in human glioma tissue and in glioblastoma cell lines such as U87MG cells. These cells exhibited malignant growth properties in culture and were tumorigenic in nude mice. When either knockdown or knockout strategies were used to deplete U87MG cells of ACSVL3, they adopted a more normal growth rate and produced significantly fewer, slower growing tumors in mice. An inhibitor of ACSVL3, if identified, could prove to be a valuable pharmacotherapeutic agent in GBM. Therefore, we sought to identify small molecule compounds that decrease or block the enzyme activity of ACSVL3, as measured by the formation of stearoyl-CoA from the 18-carbon saturated fatty acid stearic acid, a preferred substrate for ACSVL3. We approached this in two ways. First, we tested several compounds that were previously shown to inhibit the activity of a structurally and functionally related enzyme, ACSVL1. Several compounds tested showed inhibition of stearoyl-CoA formation in U87MG cells when added to an in vitro enzyme assay. These included drugs triflupromazine, phenazopyridine, chlorpromazine, emodin, and perphenazine which are approved for treating other conditions. Also inhibitory to stearoyl-CoA production were several compounds from a ChemBridge Corporation library designated CB2, CB5, CB6 and CB 16.2. One caveat regarding interpretation of these results is that in addition to ACSVL3, all cells including U87MG contain other acyl-CoA synthetases capable of using stearic acid as substrate. Therefore, we also measured stearoyl-CoA synthetase activity in ACSVL3-deficient U87MG cells (U87-KO). If a drug or compound is an ACSVL3 inhibitor, it should decrease total conversion of stearate to stearoyl-CoA more in U87MG than in U87-KO cells. By this criterion, most of the tested compounds showed some ACSVL3-specific inhibition. At the screening concentration of 80μM drug, CB5 and CB16.2 showed the greatest potency to inhibit ACSVL3 enzyme activity; at 10 μM, CB5 still showed significant inhibition but CB16.2 did not. We conclude that these compounds are worthy of further investigation as potential therapeutic agents in GBM, but additional drugs that have greater specificity and are effective at significantly lower concentrations must also be identified. Therefore, our second strategy was to develop a high-throughput library screening assay. For this, we took advantage of the fatty acid transport capability of some ACSVL family members. ACSVL1, when heterologously expressed in COS-1 cells, promotes cellular uptake of the fluorescent fatty acid analog C -BODIPY-C ; in contrast, overexpressed ACSVL3 does not. We used a domain-swapping strategy to replace the N-terminal 210 amino acids of ACSVL3 with the N-terminal 100 amino acids of ACSVL1, producing ACSVL1/3. Unlike ACSVL3, ACSVL1/3 robustly promoted C -BODIPY-C uptake while retaining the catalytically active C-terminus of ACSVL3. Most of the drugs and compounds that decreased stearoyl-CoA synthetase inhibition also inhibited C -BODIPY-C uptake in a concentration-dependent manner. Catalytically defective ACSVL1/3 mutants lost their ability to promote C -BODIPY-C uptake. Thus, we conclude that chimeric ACSVL1/3 gained the fatty acid transport function of ACSVL1 while retaining the catalytic properties of ACSVL3. A pilot screening study of >1280 drugs from an approved drug library and >880 compounds from a library of drugs predicted to cross the blood-brain barrier detected more than 50 molecules that lowered C -BODIPY-C by more than 3 standard deviations. Although secondary screening will likely exclude many or all of these, our findings support the notion that we have developed a viable method for detecting potential ACSVL3 inhibitors. Further characterization may reveal candidate pharmacologic agents for treatment of GBM and other cancers.
脑肿瘤,尤其是多形性胶质母细胞瘤(GBM),是人类最具侵袭性且最难治疗的肿瘤之一。即便采用手术、放疗和化疗相结合的方法,GBM患者的5年生存率也仅约为7%。因此,需要新的治疗方法。我们之前发现,脂肪酸代谢酶“超长链酰基辅酶A合成酶3”(ACSVL3)在人类胶质瘤组织以及U87MG细胞系等胶质母细胞瘤细胞系中过量产生。这些细胞在培养中表现出恶性生长特性,并且在裸鼠中具有致瘤性。当采用敲低或敲除策略使U87MG细胞中的ACSVL3缺失时,它们的生长速率变得更正常,并且在小鼠中产生的肿瘤显著减少且生长缓慢。如果能够鉴定出ACSVL3的抑制剂,那么它可能会成为治疗GBM的一种有价值的药物治疗剂。因此,我们试图鉴定能够降低或阻断ACSVL3酶活性的小分子化合物,通过测定从18碳饱和脂肪酸硬脂酸(ACSVL3的一种优选底物)形成硬脂酰辅酶A来衡量。我们通过两种方式来进行。首先,我们测试了几种先前已被证明能够抑制结构和功能相关酶ACSVL1活性的化合物。在体外酶测定中添加到U87MG细胞时,测试的几种化合物显示出对硬脂酰辅酶A形成的抑制作用。这些化合物包括已被批准用于治疗其他病症的药物三氟拉嗪、非那吡啶、氯丙嗪、大黄素和奋乃静。ChemBridge公司文库中的几种化合物(编号为CB2、CB5、CB6和CB 16.2)对硬脂酰辅酶A的产生也有抑制作用。关于这些结果的解释需要注意的一点是,除了ACSVL3之外,包括U87MG细胞在内的所有细胞都含有其他能够将硬脂酸用作底物的酰基辅酶A合成酶。因此,我们还测量了ACSVL3缺陷型U87MG细胞(U87-KO)中的硬脂酰辅酶A合成酶活性。如果一种药物或化合物是ACSVL3抑制剂,那么它在U87MG细胞中应该比在U87-KO细胞中更能降低硬脂酸向硬脂酰辅酶A的总转化率。按照这个标准,大多数测试化合物都表现出一定程度的ACSVL3特异性抑制作用。在80μM药物的筛选浓度下,CB5和CB16.2对ACSVL3酶活性的抑制效力最大;在10μM时,CB5仍表现出显著抑制作用,但CB16.2则没有。我们得出结论,这些化合物作为GBM潜在治疗剂值得进一步研究,但还必须鉴定出具有更高特异性且在显著更低浓度下有效的其他药物。因此,我们的第二种策略是开发一种高通量文库筛选测定法。为此,我们利用了一些ACSVL家族成员的脂肪酸转运能力。当在COS-1细胞中异源表达时,ACSVL1促进荧光脂肪酸类似物C -BODIPY-C 的细胞摄取;相比之下,过表达的ACSVL3则没有这种作用。我们采用结构域交换策略,用ACSVL1的N端100个氨基酸替换ACSVL3的N端210个氨基酸,从而产生ACSVL1/3。与ACSVL3不同,ACSVL1/3能有力地促进C -BODIPY-C 的摄取,同时保留ACSVL3具有催化活性的C端。大多数降低硬脂酰辅酶A合成酶抑制作用的药物和化合物也以浓度依赖的方式抑制C -BODIPY-C 的摄取。催化缺陷型ACSVL1/3突变体失去了促进C -BODIPY-C 摄取的能力。因此,我们得出结论,嵌合蛋白ACSVL1/3获得了ACSVL1的脂肪酸转运功能,同时保留了ACSVL3的催化特性。对来自一个已批准药物文库的1280多种药物以及来自一个预计能穿过血脑屏障的药物文库的880多种化合物进行的初步筛选研究,检测到50多个能使C -BODIPY-C 摄取降低超过3个标准差的分子。尽管二次筛选可能会排除其中许多或所有分子,但我们研究结果支持这样一种观点,即我们已经开发出一种可行的方法来检测潜在的ACSVL3抑制剂。进一步的表征可能会揭示出用于治疗GBM和其他癌症的候选药物。
