通过 A1542/3 柠檬苦素激活 ERK 可通过转录刺激胆固醇生物合成基因来减轻红细胞白血病。
ERK activation via A1542/3 limonoids attenuates erythroleukemia through transcriptional stimulation of cholesterol biosynthesis genes.
机构信息
State Key Laboratory for Functions and Applications of Medicinal Plants, Guizhou Medical University, Province Science City, High Tech Zone, Baiyun District, Guiyang, 550014, Guizhou Province, People's Republic of China.
The Key Laboratory of Chemistry for Natural Products of Guizhou Province and Chinese Academic of Sciences, Guiyang, 550014, Guizhou Province, People's Republic of China.
出版信息
BMC Cancer. 2021 Jun 9;21(1):680. doi: 10.1186/s12885-021-08402-6.
BACKGROUND
Cholesterol plays vital roles in human physiology; abnormal levels have deleterious pathological consequences. In cancer, elevated or reduced expression of cholesterol biosynthesis is associated with good or poor prognosis, but the underlying mechanisms are largely unknown. The limonoid compounds A1542 and A1543 stimulate ERK/MAPK by direct binding, leading to leukemic cell death and suppression of leukemia in mouse models. In this study, we investigated the downstream consequences of these ERK/MAPK agonists in leukemic cells.
METHODS
We employed RNAseq analysis combined with Q-RT-PCR, western blot and bioinformatics to identify and confirm genes whose expression was altered by A1542 and A1543 in leukemic cells. ShRNA lentiviruses were used to silence gene expression. Cell culture and an animal model (BALB/c) of erythroleukemia induced by Friend virus were utilized to validate effects of cholesterol on leukemia progression.
RESULTS
RNAseq analysis of A1542-treated cells revealed the induction of all 18 genes implicated in cholesterol biosynthesis. Expression of these cholesterol genes was blocked by cedrelone, an ERK inhibitor. The cholesterol inhibitor lovastatin diminished ERK/MAPK activation by A1542, thereby reducing leukemic cell death induced by this ERK1/2 agonist. Growth inhibition by cholesterol was observed both at the intracellular level, and when orally administrated into a leukemic mouse model. Both HDL and LDL also suppressed leukemogenesis, implicating these lipids as important prognostic markers for leukemia progression. Mechanistically, knockdown experiments revealed that the activation of SREBP1/2 by A1542-A1543 was responsible for induction of only a sub-set of cholesterol biosynthesis genes. Induction of other regulatory factors by A1542-A1543 including EGR1, AP1 (FOS + JUN) LDLR, IER2 and others may cooperate with SREBP1/2 to induce cholesterol genes. Indeed, pharmacological inhibition of AP1 significantly inhibited cholesterol gene expression induced by A1542. In addition to leukemia, high expression of cholesterol biosynthesis genes was found to correlate with better prognosis in renal cancer.
CONCLUSIONS
This study demonstrates that ERK1/2 agonists suppress leukemia and possibly other types of cancer through transcriptional stimulation of cholesterol biosynthesis genes.
背景
胆固醇在人体生理学中发挥着重要作用;异常水平会产生有害的病理后果。在癌症中,胆固醇生物合成的表达升高或降低与预后良好或不良相关,但潜在机制在很大程度上尚不清楚。倍半萜化合物 A1542 和 A1543 通过直接结合刺激 ERK/MAPK,导致白血病细胞死亡,并抑制小鼠模型中的白血病。在这项研究中,我们研究了这些 ERK/MAPK 激动剂在白血病细胞中的下游后果。
方法
我们采用 RNAseq 分析结合 Q-RT-PCR、western blot 和生物信息学方法,鉴定和确认 A1542 和 A1543 在白血病细胞中改变表达的基因。使用 shRNA 慢病毒沉默基因表达。利用 Friend 病毒诱导的红白血病细胞培养和动物模型(BALB/c)验证胆固醇对白血病进展的影响。
结果
A1542 处理细胞的 RNAseq 分析显示,所有 18 种参与胆固醇生物合成的基因均被诱导。Cedrelone(一种 ERK 抑制剂)阻断了这些胆固醇基因的表达。胆固醇抑制剂 lovastatin 减弱了 A1542 对 ERK/MAPK 的激活,从而减少了这种 ERK1/2 激动剂诱导的白血病细胞死亡。在细胞内水平和口服给予白血病小鼠模型时,胆固醇的生长抑制均有观察到。HDL 和 LDL 也抑制了白血病的发生,表明这些脂质是白血病进展的重要预后标志物。从机制上讲, knockdown 实验表明,A1542-A1543 对 SREBP1/2 的激活仅负责诱导一组亚组的胆固醇生物合成基因。A1542-A1543 诱导的其他调节因子,包括 EGR1、AP1(FOS+JUN)、LDLR、IER2 等,可能与 SREBP1/2 合作诱导胆固醇基因。事实上,AP1 的药理学抑制显著抑制了 A1542 诱导的胆固醇基因表达。除白血病外,胆固醇生物合成基因的高表达与肾癌的预后较好相关。
结论
这项研究表明,ERK1/2 激动剂通过转录刺激胆固醇生物合成基因抑制白血病和可能其他类型的癌症。
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