Novel Nano-Based Drug Delivery Systems Targeting Hepatic Stellate Cells in the Fibrotic Liver

Hepatic stellate cells (HSCs) exist in the liver’s perisinusoidal space, are phenotypically activated, and acquire myofibroblast-like phenotype. This phenotypic transformation is accountable for the accumulation and production of various extracellular matrix (ECM) proteins, involving different fibril-forming collagens in the perisinusoidal space, producing altered hepatic function and portal hypertension and increased vascular resistance, fibrosis, cirrhosis, and hepatocellular carcinoma. The activated HSCs/myofibroblasts are principal collagen-producing cells in the damaged liver. Therefore, fibrosis treatments are often targeting HSCs. HSCs store most of the total body’s retinol in their cytoplasm, and hence, antifibrotic nanomedicines are often targeted with vitamin A decoration. Vitamin A-decorated nanomedicines with siRNAs for transforming growth factor-beta, collagen, and connective tissue growth factors target to inhibit fibrogenesis and the ECM-associated gene expressions, leading to fibrosis regression. Similarly, a variety of miRNAs play pro- and antifibrotic function. In the fibrotic liver, the profibrotic miRNAs are targeted with their respective antagomir and the antifibrotic miRNAs are targeted with their respective agomirs along with HSC-specific nanodecoration. These miRNA treatments reduce fibrogenesis by downregulation of ECM-related gene expressions. However, liver fibrosis is caused by the upregulation of a different type of profibrotic signaling pathways associated with ECM accumulation in the fibrotic liver. Therefore, specific gene silencing by siRNAs or targeting particularly miRNA may also not effectively reduce fibrosis to a greater extent. However, nanodecoration of a drug is useful to deliver drugs into activated HSCs in the injured liver. Therefore, the aim of this review is to focus on targeted drug delivery towards activated HSCs in the persistently damaged liver.


Introduction
Chronic liver diseases are the main cause of universal health problem. Approximately, 2 million annual deaths are attributed to cirrhosis and its associated complications, hepatocellular carcinoma (HCC) and viral hepatitis [1]. Hepatic fibrosis is the common sequel of chronic liver diseases. If fibrosis is not properly treated, then it progresses into cirrhosis and its related complications like portal hypertension and HCC. Cirrhosis is considered as the most advanced stage of hepatic fibrosis. Cirrhosis and HCC rank 11 th and 16 th , respectively, in causing global deaths. Together, HCC and cirrhosis account for 3.5% of mortalities worldwide [1,2]. Liver fibrosis is caused by chronic injury due to chronic ethanol intake, hepatitis infections, and metabolic disorders [3]. Fibrosis of the liver is classically distinguished by the increased synthesis and a net accumulation of a variety of extracellular matrix, comprising collagens I, III, and V, elastin, tenascin, and fibronectin in the perisinusoidal space of the liver [4]. Thus, increased ECM synthesis and scar formation are considered as the initial event of liver fibrosis mediated by the hepatic stellate cell (HSC), which is the principal collagen-producing cell in the chronically injured liver [5]. Over the last two to three decades, our understanding of the pathophysiology of fibrosis is instrumental; several studies have identified potential antifibrotic targets either to halt progression or reverse fibrosis [6]. Chronic liver diseases are often reversible after the withdrawal of underlying etiology, and their treatment mainly focused on etiology-specific. However, presently, no accepted antifibrotic treatments are available for human use [7]. The hepatic stellate cells (HSCs) are strategically placed in the perisinusoidal area of the liver in such a way that they communicate with hepatocytes, immune cells, and sinusoidal endothelial cells in the liver. Hence, HSCs are one of the prime targets for treating fibrotic liver [8]. However, the development of natural and synthetic antifibrotic drugs targeting HSCs in the fibrotic liver has faced challenges such as poor solubility, lack of HSC-specific targeted delivery, and less effectiveness [9]. Thus, studies have principally targeted HSCs with several nanoformulations to control or regress the ongoing liver fibrosis. This review is primarily focusing on novel nano-based drug delivery systems targeting HSCs in the fibrosed liver.

Hepatic Stellate Cells
Hepatic stellate cells exist in the perisinusoidal space or Disse space in the liver. Upon chronic liver injury, HSCs are phenotypically transformed and activated into myofibroblasts. This process is termed as HSC activation [10]. The activated myofibroblasts/HSCs are liable for the expression and secretion of numerous chemokines and profibrotic cytokines [11]. Thus, activated HSCs retain the pathophysiological status of the damaged liver by expressing plateletderived growth factors (PDGF), transforming expressing growth factor-β (TGF-β), retinol binding protein (RBP) receptor, Krüppel-like factor 4, endothelin-1, and α-smooth muscle actin, modulating a variety of tissue inhibitors of metalloproteinases (TIMPs) and matrix metalloproteinase (MMPs). This process is known as perpetuation. In a normal liver, HSCs are quiescence and are liable for the preservation of normal ECM homeostasis. However, the phenotypically activated myofibroblasts or activated HSCs are liable for the accumulation and synthesis of an enormous amount of ECM to substantiate the ongoing injury of the liver [12]. Anatomically, the excessive ECM deposition in the perisinusoidal space of the chronically injured liver hinders the solute transport between hepatocytes and liver sinusoidal endothelial cells (LSECs), heading to functional alteration of the liver and an increase in intrahepatic resistancemediated portal hypertension [13]. Functionally, activated HSCs interact with several cell types in the perisinusoidal milieu by releasing PDGF, TGF-β, TIMPs, MMPs, endothelin-1, and others [14]. These signaling molecules from activated HSCs, act on themselves via an autocrine manner also activate other cells such as quiescent HSCs, hepatocytes, and LSECs via a paracrine manner. For instance, activated HSCs and LSECs communicate each other with ET-1, leading to portal hypertension [15]. Activated HSCs induce the proliferation and activation of quiescent HSCs by expressing PDGF and TGF-β, which increases the burden of ECM synthesis. The role of HSCs in the normal and injured liver is presented in Figure 1.

Existing Strategies Targeting Activated HSCs in the Fibrotic Liver
Since HSCs perform a pivotal role in fibrogenesis, several studies have targeted HSCs to regress fibrogenesis [16]. Accumulating experimental evidence suggests that the liver fibrosis process can be controlled by decreasing HSC activation and perpetuation. Previous studies have targeted HSCs for therapeutic purpose in the chronically injured liver by (i) decreasing the HSC proliferation via PDGF signaling, (ii) decreasing fibrogenesis through inhibition of TGF-β signaling, (iii) targeting HSCs to promote the ECM degradation by modulating MMPs and TIMPs, (iv) inducing the clearance of activated HSCs by apoptosis, (v) inducing senescence of activated HSCs, (vi) inhibiting the proliferation of activated HSCs by halting their cell cycle, (vii) suppressing the parenchymal and qHSC activation by removal of underlying etiologies, (viii) neutralizing the oxidative stress environment of the injured liver by using antioxidants, (ix) silencing the activated HSC genes responsible for ECM synthesis, (x) targeting the profibrotic miRNAs in activated HSCs via antagomirs, (xi) decreasing epigenetic alteration in activated HSCs, and (xii) decreasing the extracellular vesicles released from activated HSCs [17][18][19][20][21][22][23]. The above strategies were employed by previous experimental studies by using natural and synthetic drug candidates to regulate the activated HSCs in the chronically damaged liver. However, these drugs have several disadvantages like poor bioavailability and solubility, less targeted, and off-target effects on drug delivery. The liver contains heterogenous cell population, predominantly HSCs, hepatocytes, LSECs, Kupffer cells, portal fibroblasts, and other non-resident immune cells. However, HSCs activation often leads to the overexpression of several cell surface receptors such as collagen type 4, TGF-β, connective tissue growth factor receptors, PDGFRβ, RBP receptor, synaptophysin, cluster of differentiation 44 (CD44), insulin-like growth factor-II receptor (IGF2R), and low-density lipoprotein receptor [24]. In previous studies, these receptors have been primary targeted to direct nano-based drugs towards activated HSCs. Therefore, targeting phenotypically activated HSCs in the damaged liver by nano-based drug preparation could be one of the possible strategies to increase the targeted drug delivery to HSCs. Thus, HSC-specific nanodrug construction may direct the drug towards activated HSCs in the fibrosed liver.

Nanotargeting of Activated HSC Surface Proteins and Signaling
Conventionally, inorganic nanoparticles like silver, gold, titanium dioxide, silicon dioxide, and cerium oxide are used without targeting activated HSCs in the fibrotic liver [25,26]. Later, nanocarriers like liposomes and hyaluronic acid micelles are used to carry antifibrotic drugs and target HSCs in the injured liver [27,28]. These nanocarriers targetedly deliver nanoparticles into activated HSCs in the fibrotic liver. During chronic liver injury CD44 and phenotypic receptors are increasingly expressed after HSC activation. Therefore, CD44 ligands are previously targeted along with 2 Journal of Nanomaterials nanoparticles to precisely deliver numerous synthetic and natural antifibrotic agents [29]. For instance, αvβ3 integrin is greatly expressed in activated HSCs and degradation of αvβ3 ligands was found in activated HSCs during the resolution of liver fibrosis. Therefore, a previous study targeted αvβ3 on activated HSCs [30]. Hedgehog (Hh) signaling p,lays a pivotal role in the pathophysiology of liver fibrosis [24]. Hedgehog signaling components and receptors Ihh, smoothened (Smo), patched (Ptc), and glioma-associated oncogene (Gli) 2 and Gli3 were highly expressed in HSCs [31]. Sterically steady liposomes that comprise the cyclic peptides (cRGDyK) with an excessive attraction to αvβ3 were developed to attain precise delivery to activated HSCs. CRGDyK-guided liposomes were specifically adopted into activated HSCs in vivo and in vitro. However, cRGDyK-guided liposomes uptake was minimal in quiescent HSCs, Kupffer cells, hepatocytes, biliary cells, or sinusoidal endothelial cells. Vismodegib (GDC), a Hh inhibitor loaded with cRGDyK-directed liposomes, prevented Hh signaling only in activated HSCs. In vivo, GDC-loaded cRGDyK-guided liposome treatment attenduated thioacetamide induced liver fibrosis in mice or attenuated bile duct ligation (BDL) [32]. Peroxisome proliferator-activated receptor γ (PPAR-γ) overexpression prevents HSC activation in the damaged liver [33]. Rosiglitazone (RGZ), a PPAR-γ agonist, was shown to alleviate liver fibrosis via HSC activation [34]. Therefore, methoxy-polyethylene-glycol-b-poly(carbonateco-lactide) [mPEG-b-p(CB-co-LA)] was produced and encapsulated GDC and RSZ with the encapsulation efficiency being 5.0% and 2.0% w/w for GDC and RSZ, respectively, to target against BDL-caused liver fibrosis in rats. Systemic administration of drug-encapsulated nanoparticles (120-130 nm-sized) protected liver injury in BDL-induced liver fibrosis by decreasing inflammatory cytokines and controlling the activation of HSCs. GDC-and RSZ-loaded nanoparticles reduced Hh ligand molecule (Shh, Smo, Ptch-1, and Gli 1) expression and fibrosis marker expressions (α-SMA, fibronectin-1, and TGF-β1) [35]. These studies suggest that nanoparticles with Hh inhibitor and PPAR-γ agonist could target activated HSCs and reduce the fibrogenic potential. Interestingly, activated HSC integrin was targeted using plant-derived active compound quercetin and along with gadolinium. RGD-hepatitis B core (HBc)/quercetin and RGD-HBc/quercetin-gadolinium nanocages (29:6 ± 3:1 nm) were prepared with the surface-presented RGD-directing ligand. These nanocages display high binding attraction with integrin αvβ3 and thereby achieved targeted delivery towards activated HSCs. These nanocages effectively prevented the HSC proliferation and their activation in vitro. This study shows that multifunctional αvβ3-directed NPs could deliver quercetin to the activated HSCs [36]. Germacrone (GMO), a major bioactive component of Curcuma zedoaria, and miR-29b, an antifibrotic miRNA encapulated into nanoparticles based on poly(ethylene glycol)-block-poly(lactide-co-glycolide) (PEG-PLGA), were developed with cyclical RGD peptides (231.2 nm size) for an active ligand to integrin αvβ3 binding. This nanoparticle system efficiently internalized into HSCs via αvβ3-mediated endocytosis. GMO and miR-29b inhibit the proliferation of activated HSCs and collagen 1 expression, and in vivo, this nanoparticle system ameliorated CCl 4 -induced liver fibrosis in mice [37].

Vitamin A-(VA-) Coupled Nanoparticles Targeting activated HSCs
HSCs store 80% of the body's total retinol existing as retinyl esters inside their lipid droplets. Vitamin A storage is a characteristic feature of HSCs [38], and therefore, this property  has been applied as a mechanism for targeting HSCs. Most of the natural antifibrotic compounds have poor solubility and bioavailability [9]. Hence, to achieve targeted drug delivery to HSCs, VA decoration may be a useful strategy to direct the antifibrotic compounds towards activated HSCs in the damaged liver [3,39]. In a study, zein/phospholipid composite NPs coupled with VA (192 nm) were formed as a delivery platform for gallic acid (GA-CACNP/VA), a polyphenolic compound, reportedly having antifibrotic effects. These NPs showed high (60%) entrapment efficiency (EE%), selectively distributed in the liver and highly internalized into HSCs. GA-CACNP/VA evidently inhibited HSC activation, induced activated HSC apoptosis, and repressed collagen deposition [40]. This study implies that VA decoration can lead to HSC-specific efficient drug delivery in the injured liver. In a study, retinol was conjugated with polyethyleneimine, which further combined with an antisense oligonucleotide to form retinol-conjugated polyethyleneimine (RCP) nanoparticles. Retinol conjugation caused specific recruitment of retinolconnecting protein in the corona that effectively directed the nucleotide-laden nanoparticles into HSCs in the fibrotic liver. The oligonucleotide-laden RCP nanoparticles suppressed collagen 1 expression and attenuated CCl 4 -and BDL-caused liver fibrosis in mice [41]. Imatinib, a second-generation tyrosine kinase inhibitor (TKI), has been significantly employed for the treatment of HCC, gastrointestinal stromal tumors, and chronic myelogenous leukemia [42]. Imatinib was shown to inhibit TGF-β signaling and profibrotic PDGF pathways [43]. Therefore, VA-combined imatinib-rich liposomes (spherical and 71:9 ± 2:6 nm-sized) have been targeted against HSCs in the fibrotic liver in rats. The VA-coupled imatinib liposomes are acumulated in the fibrotic liver when compared to the normal liver in rats. A single intraperitoneal injection of this liposome had 13.5 folds higher hepatic accumulation. Colocalization of VA-coupled liposome-rich Nile Red with immune-fluorescently labeled PDGFRβ in frozen liver tissue sections confirmed HSC directing [44]. The acumulation of different ECM in the liver perisinusoidal space is the chief pathological feature of liver fibrosis [8]. Thus, acceleration of matrix degradation is considered one of the therapeutic strategies for fibrosis regression. In a study, collagenase I, a collagen 1-degrading enzyme, and retinol-codecorated polymeric micelle that possesses nano-drill-like and HSC target function based on poly-(lactic-co-glycolic)-b-poly(ethylene glycol)-maleimide (PLGA-PEG-Mal) (CRM) was prepared. The spherical CRM (87:6 ± 8:3 nm) had a nano-drill-like function and effectively degraded pericellular collagen I. CRM loaded with nilotinib, a second-generation TKI, showed antifibrotic activity against CCl 4 -induced liver fibrosis [45].

Nanotargeting of activated HSCs for Portal Hypertension
Increased intrahepatic resistance and portal hypertension are major complications of advanced fibrosis and cirrhosis. HSC activation and subsequent ET-1 release from myofibroblasts and LSECs cause portal hypertension [15]. The influence of angiotensin II receptor antagonist, i.e., valsartan, on portal hypertensiand hepatic fibrosis has been studied in hepatic cirrhotic patients [46,47]. Valsartan reduced portal hypertension in hepatic cirrhosis patients [48]. However, valsartan exhibits poor water-soluble (0.18 mg/ml) property and it has~23% of oral bioavailability [49]. Therefore, liposome-based nanocarriers for valsartan were developed to improve its permeability. These valsartan-loaded liposomes (VLL) (spherical and 169:9 ± 2:4 nm-sized) are coupled with VA for HSC specific targeted delivery. The orally administered VLL preferentially accumulated in the fibrotic liver for six days [50]. Further, reduced PPAR-γ nuclear receptor expression was reported during HSC activation, while its upregulation was responsible for the regression of fibrosis and downregulation of fibrosis-associated gene expressions and fibrosis resolution [33]. VLL exhibits poteintal antifibrotic effects with PPAR-γ agonistic activity and prolonged delivery [50]. Nitric oxide is a potent vasodilator, and it was shown to inhibit HSC activation and regulate portal hypertension [15]. Therefore, nitric oxide (NO) donor molecule-based drug delivery systems have been developed. For instance, silica and gold nanoparticlearbitrated drug delivery systems containing NO donors have been tried against liver fibrosis. NO released from silica and gold nanoconjugates inhibited HSC proliferation, activation, and their vascular tube formation ability [51]. Similarly, polymeric nanoparticles incorporating nitric oxide donor molecules (S-nitrosoglutathione), conjugated with VA (25-35 nm-sized), were studied in vitro and in vivo. The VA decoration led to the polymeric nanoparticles specifically target rat primary HSCs and LX-2 cells. This nanoparticle system significantly inhibited fibrogenic marker gene expressions such as collagen and α-SMA without inducing cytotoxicity in primary HSCs isolated from rats and in human HSC cell line (LX-2). Further, NO-delivering nanoparticles have reduced the ET-1 and portal pressure (approximately 20%) in BDL rats [52]. These studies indicate that gold, silver, and polymeric nanoparticle system may serve as a novel delivery platform to deliver anti-hypertensive drugs and vasodilators like NO into activated HSCs responsible for portal hypertension during chronic liver diseases.

RNA Interference-Based Targeted Drug Delivery in liver fibrosis
RNA interference is one of the valuable approaches to regress fibrosis of the liver by silenceing specific gene expression in activated HSCs [53]. The activated HSCs are liable for the accumulation of a variety of ECM proteins in the perisinusoidal space of chronically injured liver, which causes liver fibrosis. Therefore, ECM-specific gene silencing may reduce the ECM accumulation in the liver, decreasing fibrosis and associated complications [54]. siRNA-based nanopreparation offers promissing and targeted drug delivery. For instance, siRNA-mediated interference of poly(rC) binding protein 2 (PCBP2) gene inhibits the expression of α-complex protein-2 (αCP2) in HSCs, which is accountable for stabilization of collagen α1(I) mRNA. The decay rate of the collagen α1(I) mRNA was shown to increase 4 Journal of Nanomaterials significantly after streptavidin, siRNA, cholesterol, and protamine (SSCP) nano-multifaced treatment in activated HSCs [55]. Later, Shukla et al. [56] demonstrated the intracellular transferring of oligonucleotide siRNA and their effective discharge into the HSC cytosol. After internalization, the siRNA nanocomplex with protamine and streptavidin entrapped in early endosomes undergoes exocytosis, entrapment in lysosomes, and endosomal escape. This caused a substantial quantity of siRNA dissociation from the nanocomplex to utilize gene silencing activity. The IGF2R is increasingly expressed in activated HSCs. Therefore, biotin-conjugated IGF2R-specific peptide, vitamin A, and cholesterol were used as the targeting ligands for the neutravidin-based siRNA nanocomplex to deliver PCBP2 siRNA to activated HSCs. Interestingly, IGF2Rspecific siRNA-neutravidin-peptide-protamine nanocomplex (228 nm) showed a maximum targeting effect to human (LX-2) and rat (HSC-T6) HSCs and activated initial rat HSCs as compared to cholesterol (191 nm) and vitamin A (167 nm) nanocomplexes. IGF2R-specific siRNA-neutravidin-peptide-protamine nanocomplex exhibited the highest liver uptake than lung and kidney in CCl 4 -induced fibrotic rats. IGF2R-specific siRNA-neutravidin-peptide-protamine nanocomplex had maximum PCBP2 silencing and prevented the migration of activated HSCs [57]. Though siRNA-neutravidin-peptide-protamine nanocomplex possesses greater than 228 nm size due to higher molecular weight of the peptide ligand, still they achieved the maximum liver intake. Vitamin A nanocomplexes have less than 200 nm size as compared to the cholesterol based nonocoplex. However, for liver directing, the avergage particle size was defined to be less than 200 nm, which highly promotes passive liver targeting [39]. Therefore, a study from Zhao et al. [57] suggests that nanoparticles with more than 200 nm particle size also possibly target the liver.
The chitosan is a natural, recyclable and hydrophilic polymer; it is commonly used in the development of nanoparticles (NPs) for delivery of drug, particularly for nucleic acid and protein delivery [58]. Chitosan nanoparticles have an innate affinity for ECM proteins such as collagen, suggesting that they could be used to transport drugs to fibrotic livers. A previous study developed TGF-β-siRNA-loaded chitosan NPs (spherical shaped, zeta potential (ZP) of 35 ± 1 mV, and hydrodynamic diameter (HD) 110 ± 6 nm) to promote efficient delivery into activated HSCs via modification with PDGF-β binding peptides. The addition of collagenase increased the internalization of TGF-β-siRNA-rich chitosan NPs and delivered anti-TGF-β1 siRNA into activated HSCs in vitro and in vivo. Collagenase-containing nanoparticles may help to degrade the collagen-rich fibrotic scar in the  5 Journal of Nanomaterials chronically injured liver [59]. Tenascin-C (TnC), an ECM protein secreted by HSCs is minimally detected in normal liver cells; however, it is transiently expressed during tissue damage and performs an important role in tumorigenesis and fibrogenesis [60]. TnC promotes HSC activation, migration, and TGF-β-mediated type I collagen production in the chronically damaged rat liver [61]. In a study, functionalized mesoporous silica NPs (size 40 ± 5 nm; HD 157 ± 15 nm) were used for the efficient transport and delivery of siTnC in HSCs. Inhibition of TnC by mesoporous silica NP-loaded siTnC prevents HSC activation-mediated cell migration and prevents the elevation of proinflammatory gene expression in macrophages [62].
Herbal-based hepatoprotective preparations have poor solubility, bioavailability, and rapid clearance. Therefore, to increase their solubility and bioavailability, nano-based approach is commonly used in experimental studies and tested against fibrosis models [9]. The herbal-based antifibrotic drug nanopreparation may be useful to target HSCs. For instance, a previous study desinged and optimized a reverse micelle-loaded lipid nanocapsule using Box-Behnken design to deliver GA, which has antifibrotic effect, directly into activated HSCs. These 30:35 ± 2:34 nm-sized GA nanoparticles had high EE (63:95 ± 2:98%w/w) with effective internalization into activated HSCs and reduced their proliferation and induced apoptosis. In vivo, these NPs accumulated in the liver and downregulated the fibrotic marker gene expressions [67]. San-Huang-Xie-Xin-Tang decoction containing Rhei rhizome, Coptidis rhizome, and Scutellariae radix, a traditional herbal medicine of China, is extensively used as hepatoprotective treatment. These dried herbal mixtures were nanoscaled using a pulsed air flow pulverizer. These pulverized nanoscale herbal mixtures induced cytotoxicity in HSCs. This nanoherbal extract has also upregulated MMP-2 gene expression and inhibited TIMP-1 gene expression [68]. However, RNA interference using siRNA and miRNAs encounters many challenges after its systemic administration. Successful and consistent siRNA delivery to activated HSCs in the fibrotic liver remains a vital issue for the synthesis of siRNA-based therapies. The targeted drug delivery for activated HSC in the fibrotic liver is presented in Figure 2.

Conclusion and Perspectives
Undoubtedly, vitamin A-conjugated nanoparticles or siRNAs or miRNAs or drugs successfully deliver antifibrotic drugs into activated HSCs in the chronically injured liver and reduce profibrotic protein and gene expressions. Vitamin A-conjugated nitric oxide donor molecules and other antihypertensive drugs selectively deliver drugs into activated HSCs and reduce portal hypertension. To achieve better liver targeting, the average particle size was defined to be less than 200 nm, which greatly promotes passive liver targeting. However, Zhao et al. [57] developed a siRNA-neutravidin-peptide-protamine nanocomplex that achieved maximum targeted liver delivery with the particle size of 228 nm. Therefore, size is not the only factor to achieve the highest theranostic potential of a nanocomplex. Hepatic fibrosis is a consequence of the accumulation of numerous ECM proteins in the damaged liver. Therefore, targeting one protein expression via gene silencing using siRNAbased nanoconstruct may not give us efficient results and this is one of the main limitations of siRNA-based therapeutics. However, nanodecoration of HSC-specific molecules provides better siRNA delivery. Further, exocytosis is one of the main factors responsible for the transient silencing activity of non-viral siRNA delivery, and therefore, exocytosis inhibitor combination may prolong the silencing activity of siRNA. However, this approach should be studied in detail in the near future. Moreover, a variety of miRNAs are modulated during HSC activation. They have specific profibrotic and antifibrotic properties; therefore, their specific antagomir-and agomir-based nanopreparations should be studied in an eloborate manner, respectively. Thus, liveror HSC-specific nanopreparation remains a gold standard strategy to deliver siRNA/miRNA/drugs into activated HSCs in the fibrotic liver.

Data Availability
The data used to support the findings of this study are included within the article

Conflicts of Interest
The authors declare that they have no conflicts of interest.