Psoralen and Isopsoralen from Psoralea corylifolia Suppress NSCLC by Dual Mechanisms: STAT3 Inhibition and ROS Modulation
Liwei Bi, Guangyi Chen, Wanfen Liu, Anastacio T. Cagabhion, Yu-Wei Chang, Zhengyuan Yao, Jing Feng, Yi Liu, Siyi Chen, Yung-Husan Chen

TL;DR
This study shows that compounds from Psoralea corylifolia can fight lung cancer by blocking a key protein and regulating cell-damaging molecules.
Contribution
The novel contribution is identifying psoralen and isopsoralen as dual-action STAT3 inhibitors with ROS modulation in NSCLC.
Findings
Psoralen and isopsoralen bind to STAT3 with KD values of 80.92 µM and 28.11 µM.
Both compounds inhibit cancer cell proliferation and migration while scavenging free radicals.
They reduce ROS in healthy cells but increase ROS in cancer cells under oxidative stress.
Abstract
Background: Non-small cell lung carcinoma (NSCLC) is the most prevalent form of lung cancer, and its progression is closely associated with constitutive activation of signal transducer and activator of transcription 3 (STAT3). This study used surface plasmon resonance (SPR) technology to develop a STAT3-targeting recognition system and identify natural STAT3-targeting compounds from the traditional Chinese medicine Psoralea corylifolia and to evaluate their anti-NSCLC activities, with particular attention to reactive oxygen species (ROS) regulation. Methods: The SPR biosensor immobilized with STAT3 was used to screen and enrich STAT3-binding constituents of Psoralea corylifolia, and to determine ligand-STAT3 affinities. Molecular docking was performed to characterize interactions within the STAT3 SH2 domain. Functional effects were assessed in A549 cells using proliferation and scratch…
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Figure 14- —Fujian Provincial Natural Science Foundation
- —Natural Science Foundation of Xiamen
- —Natural Science program of Xiamen Medical College
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Taxonomy
TopicsCytokine Signaling Pathways and Interactions · Bioactive natural compounds · Synthesis of Organic Compounds
1. Introduction
Lung cancer stands as the primary driver of global cancer mortality. According to global statistics, approximately 1.8 million individuals succumbed to lung cancer in 2022 [1]. Non-small cell lung cancer (NSCLC) constitutes roughly 85% of all lung carcinoma diagnoses [2]. Notably, nearly two-thirds of NSCLC cases are identified at advanced stages, resulting in a 5-year net survival rate of only 15–30% [3]. Targeted therapies, especially epidermal growth factor receptor tyrosine kinase inhibitors (EGFR-TKIs), have revolutionized outcomes for patients harboring specific driver mutations. However, their long-term effectiveness is limited by several key challenges: restricted indications, treatment-related toxicities and adverse effects, and the inevitable emergence of acquired resistance [4,5]. Platinum-based chemotherapy remains the standard of care for patients lacking actionable driver mutations (approximately 50% of NSCLC cases), underscoring the urgent need to develop novel antitumor agents with high efficacy and low toxicity [6].
Signal transducer and activator of transcription 3 (STAT3) regulates genes involved in diverse physiological and pathological processes. STAT3 is constitutively activated in more than 50% of NSCLC patients [7]. As a critical driver of multiple cancers, aberrantly activated STAT3 plays a pivotal role in promoting tumorigenesis, drug resistance, and metastasis in NSCLC, with multidimensional regulatory mechanisms underlying its oncogenic activity [3] (Figure 1). STAT3 can be phosphorylated and activated by the Janus kinase family to upregulate anti-apoptotic proteins (e.g., Bcl-xL and Mcl-1), cell-cycle regulators (e.g., cyclin D1 and c-Myc), and vascular endothelial growth factor (VEGF) expression, thereby promoting tumor proliferation, survival, and angiogenesis [8]. Additionally, STAT3 encourages the expansion of myeloid-derived suppressor cells (MDSCs), inducing immunosuppression in lung cancer [9]. High STAT3 activation in the tumor microenvironment promotes the expression of epithelial-to-mesenchymal transition (EMT)-related transcription factors, including Snail, Twist, and ZEB1, which drive cancer metastasis by upregulating genes involved in metastasis [10]. Cisplatin remains the primary chemotherapeutic agent for advanced NSCLC treatment; STAT3 expression is closely associated with tumor cell sensitivity to chemotherapeutic agents. Inhibiting STAT3 activity or expression can enhance tumor cell sensitivity to chemotherapeutic agents such as cisplatin, thereby improving treatment outcomes [11]. Consequently, discovering new drugs with STAT3-inhibitory activity is crucial to improving NSCLC therapy. No direct STAT3 inhibitors have been approved for marketing, although several are currently under preclinical and clinical studies. Most small molecules (e.g., the imidazopyridine analogue W2014-S) can inhibit STAT3 dimerization or phosphorylation, but they suffer from insufficient selectivity and off-target effects [12,13]. Natural products have become a revolutionary trend in the development of anti-cancer drugs due to their multi-purpose regulatory properties and low toxicity. However, existing studies (e.g., on resveratrol and berberine) lack direct evidence of target binding [14].
Surface Plasmon Resonance (SPR) biosensors facilitate real-time, label-free monitoring of biomolecular interactions, especially in characterizing small molecule-protein binding events (e.g., determining affinity and dissociation constants) [15]. This technology has demonstrated advantages, including label-free detection, real-time monitoring capability, and high specificity. Currently, SPR technology finds essential applications in research on active ingredients derived from traditional Chinese medicine (TCM) [16]. Notably, this technique eliminates the need to pre-separate components in herbal extracts, allowing direct screening of active ingredients that interact with specific target proteins. When combined with UPLC-Q-TOF-MS/MS, it enables accurate structural characterization of binding components. Compared to conventional SPR screening methods, the SPR-automated injection and retrieval system (SPR-AIRS) offers significant advantages, including higher detection throughput, enhanced enrichment capacity, and more definitive structural information [17].
Psoralea corylifolia Linn., also known as “Fructus Psoraleae” or “Bu Gu Zhi”, refers to the dried fruits of this leguminous medicinal plant. As a traditional Chinese medicine (TCM), its earliest recorded mention appears in the ancient text “Lei Gong Pao Zhi Lun” (Eastern Han Dynasty) and was formally included in the “Tang Ben Cao” (Tang Dynasty) [18]. Its nature is pungent and bitter, warm in property, and it targets the kidney and spleen meridians. It is primarily used to treat conditions such as kidney yang deficiency-induced lumbago and knee cold pain, spermatorrhea, nocturia, frequent urination, the five fatigues and seven injuries, wind-cold disorders, and bone marrow injuries [19]. Additionally, it is widely used to manage vitiligo (leukoderma), psoriasis, and other skin conditions [20,21]. The primary chemical constituents of Psoralea corylifolia include coumarins, monoterpene phenols, flavonoids, and benzofuranes. Contemporary pharmacological studies have revealed that extracts and monomer compounds from Psoralea corylifolia possess unique therapeutic effects against infectious diseases, inflammatory disorders, tumors, and depression [22,23]. Recent findings indicate that the active compounds of Psoralea corylifolia demonstrate significant inhibitory and therapeutic effects on malignant tumor cells, including hepatocellular carcinoma [23], breast cancer [24], prostate cancer [24], colorectal cancer [25], gastric cancer [26], and lung cancer [27]. This echoes the aberrant STAT3 activation observed in malignant tumors. Current research has also primarily focused on the regulation of classical pathways, such as epidermal growth factor receptor (EGFR), by Psoralea corylifolia components. In contrast, the direct mechanistic intervention on the STAT3 signaling pathway remains unclear [28]. Investigating whether small molecules from Psoralea corylifolia exert antitumor effects by targeting STAT3 could not only deepen research on TCM modernization but also provide novel strategies for developing natural-origin STAT3 inhibitors [29].
Reactive oxygen species (ROS) are critically involved in the progression of multiple cancer types, across various malignancies, particularly by driving tumorigenesis through oxidative damage to intracellular lipids, proteins, and DNA, which can lead to genomic instability [30]. Within the tumor microenvironment, elevated ROS levels function as signaling molecules to activate oncogenic pathways (e.g., the ERK signaling pathway), thereby promoting cancer cell proliferation, angiogenesis, and metastasis [31]. Additionally, ROS exhibit a complex regulatory relationship with STAT3, acting as upstream activators that modulate STAT3 signaling [32]. These observations suggest that compounds capable of simultaneously targeting STAT3 and modulating ROS homeostasis may exert enhanced and selective anticancer effects.
Given the critical role of STAT3 in NSCLC, this study used the SPR-AIRS system to identify small-molecule ligands targeting STAT3 proteins from Psoralea corylifolia. Molecular docking was employed to characterize their binding modes within the STAT3 SH2 domain, followed by in vitro assays to evaluate their effects on NSCLC cell proliferation, migration, and redox regulation. By integrating target-based screening with functional validation. This study aims to establish a systematic strategy for the discovery of natural STAT3 inhibitors and to elucidate the mechanisms underlying their anti-NSCLC activity. The experimental flow is depicted in Figure 2.
2. Results
2.1. Coupling Results of STAT3 Protein
To establish a reliable STAT3-based SPR screening platform, optimal immobilization conditions for STAT3 immobilization on the CM5 chip were identified as 10 mM sodium acetate at pH 4.0 and a STAT3 concentration of 50 μg/mL. Under these conditions, the ligand coupling channel yielded a robust RU value of 12,000 RU (Figure 3A). This coupling level is adequate for subsequent experiments.
2.2. Validation of STAT3 Protein Chip Specificity
To evaluate the specificity and performance of the STAT3-immobilized sensor chip, binding affinity analysis was conducted using Stattic, a well-characterized small-molecule STAT3 inhibitor. Affinity analysis revealed a KD of 46.14 μM for Stattic with the STAT3 protein (Figure 3B). KD values are inversely correlated with binding affinity; lower KD values indicate stronger binding between a small molecule and its target protein. Typically, KD values for drug-grade small molecules binding to target proteins range from nM to μM. The KD value of 46.14 μM for Stattic in this study falls within this range. Therefore, Stattic can serve as a positive control for screening herbal compounds.
2.3. SPR Screening of STAT3-Binding Components from Psoralea corylifolia
SPR screening was performed to assess the binding activity of Psoralea corylifolia extracts toward STAT3. Both 60% and 90% ethanol extracts of Psoralea corylifolia at 100 μg/mL showed binding activity to the STAT3 protein, with the 90% extract exhibiting stronger interaction (response values of 20.7 RU and 24.1 RU, respectively). It is generally accepted that a response value exceeding 20 RU, after subtracting the reference channel [31], indicates specific binding. Further concentration-dependent experiments confirmed that the response values of the psoralen 90% ethanol extract increased with concentration on the protein chip (Figure 4). This behavior clearly indicates that the extract contains bioactive components that specifically bind to STAT3.
2.4. UPLC-Q-TOF-MS/MS Analysis and Identification
The 90% ethanol extract of Psoralea corylifolia was injected into the SPR system using high-affinity coupling to STAT3 protein, aiming to recover the components enriched on the chip. UPLC-Q-TOF-MS/MS was used to analyze and identify both the extract and the recovered samples. The Base peak index/chromatogram (BPI) of the recovered sample is shown in Figure 5A. The same ion signal peaks were identified in both the Psoralea corylifolia extract and its recovered sample, as shown in Figure 5B,C (Rt = 2.94 min, m/z = 187.0400 ([M + H]+)). The compound was queried as psoralen, and its tautomer, isopsoralen, was retrieved from the ChemSpider Data Sources database. The ion signal peaks of psoralen and isopsoralen standards under the same conditions are shown in Figure 5D (Rt = 2.94 min, m/z = 187.0400 ([M + H]+)). The detailed identification of the compounds is presented in Table 1. (See Figures S1–S3 and Table S1 for additional TIC/BPI data and compounds information)
2.5. Validation of Affinity Between STAT3 Protein and Candidate Compounds
To verify whether psoralen and isopsoralen were directly bound to STAT3 protein, the affinity between both compounds and STAT3 was measured using a SPR assay. The results demonstrated stable, concentration-dependent binding signals between psoralen, isopsoralen, and STAT3 protein. The sensing signal graph and fitting curve for psoralen and STAT3 protein are depicted in Figure 6A, with a KD value of 80.92 µM, and those for isopsoralen and STAT3 protein are shown in Figure 6B, with a KD value of 28.11 µM. These results indicate that psoralen and isopsoralen bind specifically to STAT3.
2.6. Molecular Docking
The SH2 domain, a critical binding site for numerous non-peptide STAT3 inhibitors, contains three sub-pockets on its surface: the crucial phosphorylated Tyr705-specific binding pocket (pY pocket, residues Lys591, Arg609-620), the Leu706 subpocket (pY + 1 pocket, residues 626–639), and the hydrophobic side pocket (pY-X pocket, residues 592–605), where the pY pocket exhibits the highest affinity [32]. Thus, the STAT3-SH2 domain protein (amino acid positions 586–685) was selected for docking with the candidate compounds and the positive control, Stattic.
The docking results of Stattic with the SH2 domain of STAT3 protein are presented in Figure 7A. Stattic forms hydrogen bonds with residues Lys591, Arg609, and Ser636, and alkyl hydrophobic interactions with Pro639, yielding a CDOCKER binding affinity of −23.494 kJ/mol. As shown in Figure 7B, psoralen forms cation-π interactions with Lys591, hydrogen bonds with Arg609, π-hydrophobic interactions with Val637, and alkyl hydrophobic interactions with Pro639, with a CDOCKER binding affinity of −18.6669 kJ/mol. Figure 7C shows the results for isopsoralen, which forms a cation-π interaction with Lys591, a hydrogen bond with Arg609, and an alkyl hydrophobic interaction with Pro639, resulting in a CDOCKER binding affinity of −20.9622 kJ/mol. Molecular docking reveals that both compounds establish strong hydrogen bonds within the pY pocket, indicating beneficial affinity for the SH2 domain of the STAT3 protein.
2.7. Proliferation Inhibitory Effects of Psoralen and Isopsoralen on A549 Cells
The effects of psoralen and isopsoralen on the proliferation of A549 NSCLC cells were evaluated. Different concentrations of these compounds were applied to A549 cells. Absorbance values were measured to calculate cell survival rates, and IC50 values were 94.50 μM for psoralen and 260.2 μM for isopsoralen (Figure 8A–D). Results demonstrated that psoralen exhibited the most potent inhibitory effect among the compounds. Significant differences were also observed between treatment groups and the blank control group (p < 0.01), with cell survival rates decreasing in a concentration-dependent manner.
2.8. The Inhibitory Effect of Psoralen and Isopsoralen on A549 Cell Migration Using Scratch Assay
The impact of psoralen and isopsoralen on A549 cell migration was assessed using a scratch wound-healing assay. Based on proliferation assay results, concentrations of 100 μM for psoralen and 200 μM for isopsoralen were selected. The wound-healing assay was performed using concentrations close to or below the IC_50_ values to minimize nonspecific cytotoxic effects, allowing assessment of cell migratory capacity rather than cell viability. Migration areas were compared at 0, 24, and 48 h between the blank group and the treated groups. Images were captured at these time points, and migration rates were calculated to determine significant differences. Results indicated that both compounds inhibited A549 cell migration (Figure 9A). At 24 h and 48 h, 200 μM isopsoralen showed the most significant inhibition (p < 0.001), while psoralen at 100 μM also significantly reduced migration rates (Figure 9B,C).
2.9. Extracellular Antioxidant Activity of Psoralen and Isopsoralen
The antioxidant capacities of psoralen and isopsoralen were first evaluated using hydroxyl radical scavenging and superoxide anion scavenging assays. As shown in Figure 10A, the hydroxyl radical scavenging assay using the salicylic acid method showed 82.44% and 76.04% scavenging rates for psoralen and isopsoralen, respectively, indicating potent hydroxyl radical scavenging activity for both compounds. Subsequently, in the superoxide anion scavenging assay (Figure 10B), psoralen demonstrated a scavenging rate of 29.43%, while isopsoralen showed a rate of 25.38%, highlighting their ability to eliminate superoxide anions effectively. These experimental findings confirm significant antioxidant properties in psoralen and isopsoralen.
2.10. Effects of Psoralen and Isopsoralen on Intracellular ROS Levels
The effects of psoralen and isopsoralen on ROS modulation were investigated in normal HUVECs (Figure 11A) and lung cancer A549 cells (Figure 11B). In a hydrogen peroxide-induced oxidative stress model, pretreatment with psoralen and isopsoralen significantly reduced ROS levels in HUVECs (p < 0.01), indicating a protective effect against oxidative stress. Specifically, psoralen and isopsoralen decreased ROS levels in HUVECs by 73.00% and 78.63%, respectively, compared with the H_2_O_2_-treated group. In contrast, pretreatment with psoralen and isopsoralen increased intracellular ROS levels in A549 cells (p < 0.05). ROS levels were elevated by 101.10% and 75.86%, respectively, compared with the H_2_O_2_-treated group, suggesting enhanced oxidative stress that may contribute to ROS-mediated cellular damage.
2.11. Effects of Psoralen and Isopsoralen on HUVECs Proliferation
HUVECs are primary cells isolated from umbilical cord veins and are sensitive to drugs, making them a standard tool for cytotoxicity testing. In this study, psoralen and isopsoralen were applied to HUVECs at 500 μM to investigate their effects on normal cell proliferation (Figure 12A). Compared with the blank control group, neither psoralen nor isopsoralen at 500 μM significantly affected HUVECs, indicating low cytotoxicity toward endothelial cells at the tested concentration.
2.12. Effects of Psoralen and Isopsoralen on RAW264.7 Cell Proliferation
RAW264.7 cells, commonly used to model human immune responses, were treated with 500 μM of psoralen or isopsoralen. Compared to the control group, both compounds significantly increased the survival rate of RAW264.7 cells, with increases of 85.33% and 75.00%, respectively (p < 0.01). These results indicate that they do not exert cytotoxic effects on immune cells under the experimental conditions. (Figure 12B).
3. Discussion
In this study, for the first time, the STAT3-specific small-molecule inhibitors psoralen and isopsoralen from Psoralea corylifolia were identified, using SPR-AIRS technology. These compounds effectively inhibited the proliferation and migration of NSCLC A549 cells, exhibiting a selective anticancer profile and unique regulation of cellular redox status.
STAT3, as a key transcription factor, plays a central role in the onset, progression, metastasis, drug resistance, and immune escape of NSCLC [33,34]. Its sustained activation (constitutive or aberrant) is an essential feature of NSCLC and is closely associated with poor prognosis and chemoresistance [10]. Therefore, targeted inhibition of the STAT3 signaling pathway is considered a promising therapeutic strategy for NSCLC. However, the development of efficient and specific direct STAT3 inhibitors remains a significant challenge, largely due to the absence of well-defined druggable pockets and concerns regarding off-target effects [35].
SPR-AIRS technology provides an efficient and reliable screening platform for STAT3-targeted compounds [36]. It offers higher target specificity than traditional cellular phenotypic screening, enabling direct identification of active ingredients from complex herbal extracts and real-time verification of binding affinity. We first screened two specific STAT3 small-molecule inhibitors, psoralen and isopsoralen, from Psoralea corylifolia. SPR results demonstrated that both compounds bound STAT3 directly and efficiently. Molecular docking analysis further revealed that psoralen and isopsoralen explicitly bound to the SH2 domain of STAT3, a functional domain critical for dimerization and activation. This mechanism is similar to that of known STAT3 inhibitors (e.g., Stattic) [37], suggesting that psoralen and isopsoralen may inhibit STAT3 transcriptional activity by blocking its phosphorylation. These findings provide mechanistic evidence supporting STAT3 as a molecular target of psoralen and isopsoralen.
Previous studies have reported the anticancer potential of Psoralea corylifolia extracts and its constituent compounds in a variety of malignancies, including lung cancer [38]. However, most of these studies primarily focused on indirect regulatory pathways or phenotypic outcomes without demonstrating direct target engagement. By contrast, the present work establishes a clear molecular link between psoralen/isopsoralen and STAT3, and both compounds significantly inhibited the cell growth and migratory capacity of A549 lung carcinoma cells.
Notably, psoralen exhibited a more potent anti-proliferative effect despite its lower STAT3 binding affinity compared to isopsoralen. This apparent discrepancy suggests cellular responses are not solely determined by binding affinity, but rather by the integration of multiple mechanisms, including intracellular signaling modulation and redox regulation. Such divergence between biochemical affinity and cellular efficacy is commonly observed for small-molecule inhibitors and underscores the importance of functional validation beyond target-binding studies.
ROS are increasingly recognized as key regulators of cancer cell fate, functioning as both tumor-promoting signaling mediators and inducers of oxidative damage [39]. In the present study, psoralen and isopsoralen exhibited notable free radical scavenging activity in cell-free systems and effectively reduced ROS accumulation in normal HUVECs under oxidative stress conditions, suggesting a cytoprotective antioxidant effect. Conversely, in A549 cancer cells, they triggered significant ROS accumulation, exacerbating oxidative stress and suppressing proliferation. Accumulating evidence suggests that STAT3 plays a critical role in maintaining redox homeostasis in cancer cells. A reciprocal regulatory loop exists between STAT3 signaling and cellular redox homeostasis. Inhibition of STAT3 may impair antioxidant defenses, thereby promoting ROS accumulation in cancer cells, while elevated ROS can further suppress STAT3 activity [40]. In A549 lung cancer cells, STAT3 promotes cell survival and enhances antioxidant defense mechanisms [41]. Therefore, we hypothesize that suppression of STAT3 activation by psoralen and isopsoralen disrupted cellular redox balance, resulting in elevated intracellular ROS levels. In addition, modulation of ROS levels within the tumor microenvironment has been reported to reshape immunosuppressive conditions and promote antitumor immune responses [39]. Thus, the ability of psoralen and isopsoralen to regulate ROS may not only contribute to their direct cytotoxic effects on tumor cells but also potentially influence tumor-immune interactions, further enhancing their anticancer efficacy.
It should be acknowledged that the present study has certain limitations. The biological activities of the crude Psoralea corylifolia extract were not directly compared with those of the isolated compounds. Herbal extracts may exhibit synergistic effects arising from multiple constituents, and future studies will aim to systematically compare extract-level and monomer-level activities. In addition, future work should focus on in vivo validation and further elucidation of the STAT3-ROS-associated signaling cascade, including phosphorylation status, nuclear translocation of STAT3, and regulation of downstream targets such as Bcl-xL and cyclin D1, to strengthen the mechanistic understanding of these compounds.
4. Materials and Methods
4.1. Major Materials
STAT3 protein was ordered from WuXiAppTec (Shanghai, China). CM5 microarray, amino-coupling kit, 50 mM sodium hydroxide solution, glycine hydrochloride (pH 3.0), and sodium acetate (pH 4.0) were obtained from GE Healthcare (Chicago, IL, USA). Psoralea corylifolia, a traditional Chinese medicine, was provided by Associate Prof. Wang Qing from the Xiamen Key Laboratory of Traditional Chinese Medicine Bioengineering. Psoralen and isopsoralen standards were ordered from Orileaf (Shanghai, China). Ammonium bicarbonate was purchased from Merck Sigma-Aldrich (Burlington, MA, USA). NSCLC cells (A549), human umbilical vein endothelial cells (HUVECs), and RAW264.7 cell lines were obtained from the Chinese Academy of Sciences (CAS) Cell Bank (Shanghai, China). The Cell Proliferation-Toxicity Assay Kit (CCK-8) was purchased from Biosharp (Hefei, China). Stattic was ordered from TargetMol (Shanghai, China). The ROS assay kit was ordered from Beyotime (Shanghai, China).
4.2. Immobilization of STAT3 Protein on SPR Sensor Chip
SPR experiments were performed on a Biacore T200 system (GE Healthcare, USA) to immobilize STAT3 onto a CM5 sensing chip surface using the standard amine coupling protocol, with channels 2 or 4 serving as the detection pathway for STAT3 protein coupling. Initially, a 1:1 mixture of 1-Ethyl-3-(3-dimethylaminopropyl) carbodiimide (EDC) and N-hydroxysuccinimide (NHS) was introduced at a flow rate of 10 μL/min for 10 min to activate the carboxyl groups on the dextran matrix surface. Subsequently, the STAT3 protein prepared at 50 μg/mL in 10 mM Acetate buffer (pH 4.0) was delivered at 10 μL/min for 7 min to facilitate covalent conjugation. Finally, residual active groups were blocked by injecting ethanolamine. The immobilization level was quantified by measuring the bound Response Units (RU).
4.3. Examination of STAT3 Protein Chip Specificity
To validate the reliability of the experimental system, Stattic—a well-characterized small-molecule inhibitor of STAT3 was employed as a positive control [30]. At the same time, phosphate-buffered saline (PBS) served as the negative control. A serial dilution of Stattic was prepared in running buffer, and the kinetics/affinity experimental template was selected for affinity measurements. The Stattic concentration gradient was then analyzed at 25 °C with the following parameters: 60 s injection time, 30 μL/min flow rate, and 60 s dissociation time. The binding signals were specifically analyzed using reference-channel subtraction and blank subtraction. Data were fitted to a 1:1 steady-state affinity model, from which the equilibrium dissociation constants (KD) were directly derived to characterize the binding affinity between Stattic and STAT3 protein.
4.4. Preparation and Screening of Psoralea corylifolia Extract
Psoralea corylifolia was crushed and passed through a 40-mesh sieve. One gram of the powder was weighed and separately extracted with 10 mL of either 60% or 90% ethanol using ultrasonic extraction for 30 min. The extracts were then filtered through 0.22 μm syringe filters. Each filtered extract was diluted with running buffer and centrifuged to obtain the supernatant. The Biacore T200 Control Software (version 3.2.2) was launched, and the manual mode was selected. Then, Psoralea corylifolia extract was injected over the sensor chip surface for an association phase of 60 s, followed by a dissociation phase of 60 s, and then regenerated for 60 s. PBS buffer was injected between sample injections as a negative control to determine specific binding of the extract to immobilized STAT3 protein.
4.5. Recovery of Active Ingredients Bound to STAT3 Protein
To recover STAT3-bound components, all four channels of a CM5 chip were immobilized with STAT3 protein. The flow rate was then set to 10 μL/min and the binding time to 420 s. Sample angling experiments were performed using the “inject and recover” method with 10 recovery cycles, employing 0.5% trifluoroacetic acid (TFA) as the regeneration solution and 50 mM NH_4_HCO_3_ as the deposition solution. After which, all recovered solutions were combined, dried under nitrogen, redissolved in methanol, and centrifuged. The supernatant was filtered and transferred to a liquid chromatography vial.
4.6. UPLC-Q-TOF-MS/MS Analysis and Affinity Validation
The recovered samples from Section 4.5 and the corresponding Psoralea corylifolia extracts (dried and adjusted to 100 mg/mL in methanol) were analyzed using Acquity UPLC H-Class Plus Xevo Tof (Waters, Milford, MA, USA). Chromatographic conditions were as follows: Mobile phase A was 0.1% formic acid in water; mobile phase B was 0.1% formic acid in acetonitrile; gradient elution: 0–0.5 min, 10% B; 0.5–1.0 min, 10–70% B; 1.0–4.5 min, 70–100% B; 4.5–5.5 min, 100% B; 5.5–6.5 min, 100–10% B; 6.5–7.0 min, 10% B. Column temperature was maintained at 30 °C, flow rate adjusted to 0.3 mL/min, and injection volume set to 1 µL. Following the analysis, compounds in Psoralea corylifolia extracts that potentially bind to STAT3 protein were identified using Progenesis QI version 2.1 software by querying the ChemSpider Data Sources database for chemical information.
Psoralen and isopsoralen were separately diluted using the running buffer to generate multiple concentration gradients. These gradient samples were then employed to assess the binding affinity for STAT3 proteins, as described in Section 4.3.
4.7. Molecular Docking Analysis
To investigate the potential specific binding of candidate small molecules to the active site of the STAT3 protein, molecular docking was employed to assess the interactions of psoralen and isopsoralen with the SH2 domain of STAT3. The SH2 domain serves as a dimerization module and key binding site for numerous non-peptidyl STAT3 inhibitors. It functions as a critical adaptor protein, facilitating STAT3 dimerization upon activation, mediating interactions between activated receptors and downstream signaling molecules, thereby promoting pathway activation. This signaling cascade plays a critical role in the pathogenesis of NSCLC. Therefore, the SH2 domain of STAT3 was selected as the target for molecular docking with the candidate ligands (psoralen and isopsoralen) and the established STAT3 SH2 inhibitor, Stattic (used as a positive control).
The crystal structure of STAT3 was obtained from the Protein Data Bank under accession ID 1BG1. Optimization was performed using BIOVIA Discovery Studio 2019 (DS) software (v19.1.0) to remove DNA strands and water molecules, and the STAT3-SH2 domain (residues 586–685) was selected as the docking site, with a 10 Å radius. The molecular structures of the two candidate compounds, stattic and isostatticin, were obtained from the Traditional Chinese Medicine Systematic Pharmacology Database and Analysis Platform (TCMSP). Protein-receptor docking was carried out using the CDOCKER module in DS software. Stattic was used as a positive control alongside the candidate compounds, and the optimal conformation was determined by CDOCKER binding energy.
4.8. A549 Cell Proliferation Assay
A549 cells in log-phase growth were plated into 96-well plates at a density targeted to reach approximately 70–80% confluence overnight. Candidate compounds at concentrations of 0, 10, 25, 50, 100, and 200 μM were added to the A549 cells. 10 μL of the corresponding drug solution was added per well, and the plates were incubated for 24 h. After incubation, the medium was discarded, and 90 μL of fresh medium, along with 10 μL of 3-(4,5-Dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide (MTT) solution (5 mg/mL), was added to each well. The plate was incubated for four hours. The medium was subsequently discarded, and 100 μL of crystal violet dissolving solution was added to each well. The plates were shaken for 15 min. and absorbance was measured at 570 nm using a microplate reader (Biotek, Winooski, VT, USA).
4.9. A549 Cell Scratch Experiment
The cell scratch assay was used to evaluate the effect of candidate compounds on A549 cell migration [42]. Log-phase A549 cells were seeded in 6-well plates to attain 90–100% confluence by the following day. Using a marker pen and a straightedge, lines were scribed on the plate surface. Wounds were created by scratching with a P200 pipette tip to ensure uniformity. The wells were then washed twice with PBS. Subsequently, the drug solution was added at a concentration near the IC_50_ (as determined from the MTT experiment). The cells were treated with STAT3 small-molecule inhibitors and incubated. Images were captured at 0, 24, and 48 h of culture using a fluorescence inverted microscope (Leica, Düsseldorf, Germany). The scratch wound areas were quantified using ImageJ version 1.48 software (version 1.48). The cell migration rate was calculated based on wound closure as follows:
4.10. Hydroxyl Radical Scavenging Capacity Assay
The salicylic acid method was used to determine the hydroxyl radical scavenging capacity of candidate compounds [43]. The reaction system consisted of 100 µM psoralen or isopsoralen, 6 mM FeSO_4_, and 6 mM H_2_O_2_, with each component added at a volume of 50 µL in a 96-well plate. The mixture was incubated for 10 min at room temperature. Subsequently, 50 μL of 6 mM salicylic acid prepared in ethanol was added, followed by incubation at room temperature for 30 min, avoiding light. The absorbance was measured at 510 nm, and the value was recorded as A_1_. For the controls, the assay was performed identically; however, the sample was replaced with water to determine the absorbance value (recorded as A_0_), and the H_2_O_2_ solution was replaced with water to determine the absorbance value (recorded as A_2_). The clearance rate was calculated following the formula:
4.11. Superoxide Anion Scavenging Capacity Assay
The superoxide anion scavenging capacity of psoralen and isopsoralen was quantified using a modified pyrogallol autoxidation assay [44]. One hundred μL of 100 μM psoralen or isopsoralen solution was thoroughly mixed with 450 μL of Tris-HCl buffer (0.1 M, pH 8.2) and maintained at room temperature for 20 min. Then, 50 μL of 2.5 M pyrogallol was added to initiate the reaction. After 5 min of reaction, 100 μL of 0.8 M HCl was added immediately to terminate the process. Absorbance was subsequently measured at 325 nm and recorded as A_1_. For control experiments, a blank control (A_0_) was prepared by replacing the sample solution with an equal volume of water, and a background control (A_2_) was prepared by replacing the pyrogallol solution with an equal volume of water. The clearance rate was calculated following the formula:
4.12. Intracellular ROS Level Assay
Intracellular ROS levels were measured following treatment of human umbilical vein endothelial cells (HUVECs) and A549 cells with the candidate compounds to assess their effects and potential selectivity against H_2_O_2_ stress. HUVECs and A549 cells were plated separately in 96-well black plates. Following overnight culture, cells in the experimental groups were treated with serum-free medium containing 100 μM of either psoralen or isopsoralen. After 24 h of incubation, cells were washed with PBS. Then, cells from both experimental and control groups were exposed to serum-free medium supplemented with 500 μM H_2_O_2_ for four hours to induce oxidative stress. Intracellular ROS were then labeled with DCFH-DA, as instructed in the manufacturer’s ROS assay kit. Fluorescence was subsequently measured using a fluorescence microplate reader.
4.13. HUVECs Cytotoxicity Assay
HUVECs in log-phase growth were plated in 96-well plates at 1.5 × 10^4^ cells/well, with six replicate wells designated for each experimental group. After culturing for 24 h, the culture medium was carefully aspirated and replaced with 100 μL of fresh medium containing candidate compounds at 500 μM, and the culture was incubated for an additional 24 h. Subsequently, 10 μL CCK-8 solution was added to each well and incubated for 30 min before the optical density was measured at 450 nm.
4.14. RAW264.7 Cytotoxicity Assay
The murine macrophage cell line RAW264.7 in log phase was plated at 5 × 10^5^ cells/well in 96-well culture plates. After a 24-h incubation, the culture medium was aspirated and replaced with 100 μL of fresh medium supplemented with test compounds (500 μM final concentration). After an additional 24-h treatment period, 10 μL CCK-8 solution was added to each well and incubated for 30 min before optical density was measured at 450 nm.
4.15. Statistical Analysis
All experiments were performed in triplicate (n = 3) unless otherwise stated. Data are presented as mean ± SD. Statistical analyses were explicitly conducted with GraphPad Prism 8.0 software. One-way ANOVA was used to compare groups, with p < 0.05 as the threshold for statistical significance; figures were created with Origin version 2025b software.
5. Conclusions
This study provides the first direct identification of psoralen and isopsoralen derived from Psoralea corylifolia as STAT3-binding small molecules, supported by SPR-based target engagement data rather than indirect phenotypic inference. The integration of SPR-AIRS “inject-and-recover” screening with UPLC-Q-TOF-MS/MS enables direct target-oriented identification of bioactive compounds from a complex herbal matrix. Together with STAT3 binding, ROS modulation, proliferation inhibition, and the migration-suppressive effects suggest that these compounds exert multifaceted regulatory effects on NSCLC cell behavior. Their activity stems from a combination of direct STAT3 interaction and context-dependent, bidirectional modulation of ROS. The differential redox regulation, acting as an antioxidant in normal cells but a pro-oxidant in cancer cells, underscores its selective anticancer mechanism. Collectively, these findings identify psoralen and isopsoralen as early-stage STAT3-targeting bioactive compounds and underscore the utility of SPR-based target-oriented screening as an effective approach for discovering functional natural products from complex botanical sources.
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