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Key points
Chronic hepatitis B affects an estimated 240 million people worldwide.
Current treatment includes the use of nucleoside analogue inhibitors and interferons which can control virus replication but are not curative.
Several novel therapeutic strategies are in development. These include immunotherapy, gene‐editing technology and small molecule inhibitors that target the viral capsid and cccDNA.
These novel therapies aim to provide a functional cure for chronic hepatitis B.
1 INTRODUCTION
Chronic HBV infection affects around 240 million people worldwide (Figure 1A) and long‐term risks such as cirrhosis and hepatocellular carcinoma (HCC) account for approximately 600 000 deaths annually.1 HCC is one of the most frequent cancers in Africa and Asia and fibrosis is the most important prognostic predictor of survival.2 Despite the availability of several FDA‐approved drugs (Figure 1B), continuous treatment is necessary for virus replication control. Therefore, current HBV research and development programmes aim to achieve a curative strategy that either eliminates or permanently silences HBV infection. This review will discuss approved therapies and will review novel therapeutic agents currently in development.
Figure 1
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Global distribution of HBV and current therapies. (A) Worldwide distribution of chronic HBV infection. (B) Approved therapies for chronic HBV infection: ETV (entecavir), PEG‐IFN (pegylated‐interferon), TDF (tenofovir), LAM (lamivudine), LdT (telbivudine), TAF (tenofovir alafenamide). (C) Long‐term lamivudine therapy leads to reduction in cirrhosis decompensation and HCC13, 14
2 HBV REPLICATION CYCLE AND THERAPEUTIC TARGETS
HBV belongs to the hepadnaviridae family of viruses. Similar to other related species such as duck hepatitis virus and woodchuck hepatitis virus, the relatively small genome of HBV consists of a 3.2 kb partially double‐stranded DNA, referred to as relaxed circular DNA (rcDNA). HBV infects hepatocytes through a recently identified human sodium taurocholate cotransporting polypeptide (hNTCP) receptor.3 Upon fusion with the host membrane, the rcDNA‐containing nucleocapsid is released into the cytoplasm and travels to the nucleus (Figure 2). Once inside, rcDNA is converted to a highly stable episomal DNA known as covalently closed circular DNA (cccDNA) via the host DNA repair machinery molecule.4, 5 cccDNA is the transcriptional template for subsequent virus gene expression and generation of pregenomic RNA (pgRNA).6 HBV DNA is also found integrated into the host chromosome. Integration of viral DNA does not appear to play a direct role in virus replication. Instead, it is thought that HBV DNA integration may render the cellular environment more permissive to virus replication through modulating gene expression. It also likely plays an important role in hepatocellular carcinogenesis (reviewed in Ref. 7).
Figure 2
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Schematic representation of mechanisms of HBV replication and inhibition. The virus replication begins with the attachment of the virion to hepatocyte cell surface receptor hNTCP. This step can be blocked with entry inhibitors such as myrcludex B. Upon entry, the virion is released in the cytoplasm and the nucleocapsid travels to the nucleus where rcDNA enters the nucleus and cccDNA is formed. Novel cccDNA formation, or maintenance of already formed cccDNA can theoretically be disrupted with small molecule inhibitors or gene‐editing technology such as CRISPR/Cas9. Viral mRNA and pregenomic RNA are transcribed from cccDNA. Inhibition of transcription suppresses viral gene expression. HBV DNA also gets integrated into the host chromosome. Secretion inhibitors can prevent the release of HBsAg, which can be independent of the virus replication cycle. Capsid effectors/inhibitors can mislead proper nucleocapsid formation while nucleoside analogues inhibit reverse transcription inside the nucleocapsid. Secretion inhibitors can subsequently inhibit the release of enveloped virions. Finally, immunomodulators such as therapeutic vaccines and TLR agonists can enhance the immune response to chronic hepatitis B
Gene organization of cccDNA is uniquely intricate whereby several overlapping open reading frames (ORFs) code for 7 viral proteins: pgRNA serves as the template for viral polymerase‐mediated reverse transcription and subsequent synthesis of rcDNA. Another gene product of HBV is the core protein, also known as hepatitis B core antigen (HBcAg), which forms the viral nucleocapsid. Precore protein (hepatitis B e antigen, HBeAg), is a proteolytically processed viral protein that is often secreted from the infected cells and can serve as a marker for disease stage.8 Viral surface proteins, S, M and L (named based on their small, medium and large sizes respectively) are coded from the S gene whereby S is translated from S mRNA, M is translated from preS2 + S mRNA and L is translated from preS1 + PreS2 + S mRNA. All surface proteins of different length are collectively referred to as HBsAg. Finally, cccDNA also codes for viral protein X (HBx), a nonstructural protein that likely acts as a transcriptional transactivator and plays a role in regulating viral gene expression.
Once all viral proteins are synthesized and the rcDNA‐containing nucleocapsid is formed, it can travel through the cellular secretion pathway and be released as an enveloped and infectious virion. Alternatively, the nucleocapsid can cycle back to the nucleus intracellularly, whereby the recently synthesized rcDNA serves to replenish the cccDNA pool. In this way, cccDNA can be maintained even in the absence of observable viremia.9 Furthermore, cccDNA can remain dormant for a long time and only become transcriptionally activated years or decades after the initial infection. Although several therapeutic strategies have been developed against HBV replication, targeting or eliminating cccDNA, as an inert, yet highly stable mini‐chromosome has proven challenging. In this way, cccDNA elimination, or at the very least, transcriptional control, lies at the heart of the quest for a cure for chronic hepatitis B.
In theory, any step of the virus replication cycle can be a target for antiviral therapeutics (Figure 2).10 The most successful target so far has been the reverse transcription activity of pol. Interferon (IFN) treatment has also shown modest success in inhibiting virus replication. Other areas of therapeutic research include targeting of the core/capsid protein, mRNA transcription and cccDNA stability and formation. In addition to gene expression targeting technologies such as CRISPR/Cas9 and small interfering RNA (siRNA), several immune‐modulatory strategies that aim to enhance both the innate and adaptive response to CHB infection are also under investigation. The following sections will give a more detailed account of these novel strategies in development and their mechanism of action.
3 APPROVED THERAPIES FOR TREATMENT OF HBV INFECTION
The goal of CHB therapy is to improve survival by preventing risk of cirrhosis and end‐stage liver disease, and to improve quality of life.11, 12 Several therapies have been approved for CHB infection (Figure 1B). Historically, under long‐term lamivudine (LAM) treatment, HBV DNA suppression leads to reduction in cirrhosis decompensation and HCC (Figure 1C).13, 14 Thus, achieving HBV DNA clearance allows for reduction in necro‐inflammation and reduction in the risk of fibrosis progression. There are currently 2 principal therapeutic strategies approved for both HBe antigen‐positive (HBeAg+ve) and antigen‐negative (HBeAg‐ve) patients (Table 1). This includes a finite treatment course of interferon alpha (IFN‐α)/pegylated interferon (PEG‐IFN) or, a long‐term maintenance treatment with nucleoside analogues (NAs).
Table 1. Advantages and disadvantages of PEG‐IFN and nucleoside analogues
Peg‐IFN Nucleoside analogues
Advantages Finite duration High efficacy
Higher rates of HBs loss and/or seroconversion Favourable tolerability
No resistance Oral administration
Disadvantages Poor tolerability Long life duration
Moderate efficacy Unknown long‐term toxicity
Risk of adverse events Costs
Subcutaneous injection
A 1‐year treatment with PEG‐IFN offers the potential for immune control of HBV infection, with higher rates of HBeAg seroconversion and the possibility of viral suppression after stopping treatment, with loss of hepatitis B surface antigen (HBsAg) in a significant proportion of patients who maintain undetectable HBV DNA (Figure 3).15-19 However, PEG‐IFN is administered by subcutaneous injection and is associated with poor tolerability and a risk of depression. Furthermore, PEG‐IFN is contraindicated in subjects with decompensated cirrhosis, in persons with autoimmune disease and during pregnancy.
Figure 3
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HBsAg loss after therapy. Loss of HBsAg is the most reliable indicator to measure a functional cure of hepatitis B. In HBeAg(+) patients, HBsAg loss was around 11% with Peg‐IFN after 4 y, and around 10% after 5 y of TDF. In HBeAg(−) patients, HBsAg loss was still around 11% with Peg‐IFN. However, no HBsAg loss was observed after 2 y of TDF or ETV treatment15-17, 22, 23
NAs suppress HBV replication via direct antiviral activity. Usually, tolerability is good and compliance to treatment appears adequate. Entecavir (ETV) and tenofovir disoproximal fumarate (TDF) are potent HBV inhibitors with a high barrier to resistance and should be used as first‐line monotherapies. The chemical structures of various HBV reverse transcriptase inhibitors are depicted in Figure 1B.20, 21 ETV is a nucleoside analogue that disrupts DNA elongation as a delayed chain‐terminator, whereas tenofovir (TFV) is a nucleotide (adenosine) analogue that causes immediate chain termination when incorporated into HBV DNA during reverse transcription. ETV is unusual in that it is a D‐enantiomer of guanosine, and this in part accounts for its tighter binding in the active site of the enzyme as part of the mechanism of interference. Normal nucleotides can be incorporated following ETV at the 3′ hydroxyl; nevertheless, chain termination occurs shortly thereafter because of structural disruptions to the enzyme, so it is an indirect (or delayed) chain terminator, in contrast to the other agents that are used to treat HBV. TFV, in contrast, lacks a 2‐deoxyribose (cyclic) moiety including the 3′ hydroxyl group, and therefore once incorporated, it terminates polymerization. For TFV, the innovation is the use of the acyclic phosphonate group, which achieves 2 functions: (a) this group is resistant to cellular esterases that otherwise might serve to remove the phosphate group to form a nucleoside derivative, and (b) in contrast to other nucleoside analogues, this stable alteration circumvents the need for the cellular addition of the alpha phosphate, which is the rate‐limiting step in the synthesis of 2′‐deoxynucleoside triphosphates, the active substrates for reverse transcriptase.
The phosphonate group of TFV differs from a normal phosphate group in that a carbon is directly linked to the phosphorus. For a phosphate group, the phosphorus would be directly linked to an oxygen atom in place of the carbon atom in the TFV diagram above. The phosphonate is referred to as acyclic because in naturally occurring nucleotides, the phosphate group is linked to a sugar moiety (cyclic, ribose or deoxyribose), whereas this is absent in this drug. The nucleoside analogues used for HBV treatment are cyclic nucleosides (ETV, lamivudine [LAM] and telbivudine). Adefovir (ADV), in spite of its different characteristics, differs from TFV only by the lack of the methyl group (Figure 1B).
More than 95% of persons treated with the highly potent TDF and ETV achieve virological clearance. NAs are administered orally, and tolerance is good. The safety of these drugs over lifelong therapy remains to be established. Regarding the risk of drug resistance, although common in the past with earlier, less potent NAs such as LAM and ADV, resistance has become extremely rare with TDF and ETV. Long‐term clinical data up to 6 years and beyond are emerging for the newer NAs that are providing reassuring data on their efficacy and safety. There are large data that long‐term blockage of HBV replication by the most potent drugs (ETV and TDF) results in an improved long‐term survival with a decreased risk of progression to cirrhosis, end‐stage liver disease and HCC. Furthermore, a study analysing liver histology in persons treated with TDF for 5 years demonstrated fibrosis regression in the majority of patients and also cirrhosis reversal (Figure 4).22, 23 In addition, the cirrhosis reversal was observed during treatment in 75% of patients with cirrhosis, probably associated with a decreased risk of HCC and improved survival. Real‐world data with ETV and TDF in routine clinical practice are confirming the favourable safety and excellent efficacy of these therapies.
Figure 4
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Fibrosis regression under TDF. Advanced liver fibrosis and particularly cirrhosis were previously considered to be largely irreversible. Data from small studies suggest this may be possible. The histological benefits of 5 y of TDF therapy in the largest study of paired liver biopsies in HBV over 5 y of therapy are shown. The histogram shows that the proportion of patients with Ishak stages 0‐2 increased over the study period, whereas, in contrast, the proportion with Ishak stages 4‐6 decreased, thus dramatically illustrating a marked overall decrease in liver scarring for this cohort22, 23 |
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发表于 2018-8-15 20:45
