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Replies to post #194361 on Amarin Corp Plc (AMRN)
05/31/19 7:01 AM
05/31/19 7:18 AM
05/31/19 2:46 PM
06/02/19 11:03 AM
Extreme outliers due to infections caused by temporary illness or other factors can heavily influence summary statistics of hsCRP, even beyond what is handled by using a non-transformed data approach (e.g., a conventional mean or median on a nominal scale). These individual outlier results can affect a mean or median population measurement in a way that can convey a misleadingly skewed result for the population studied. For this reason, a more reliable log transformation of hsCRP is used to incorporate outlier data appropriately within the context of the entire data set.
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Eligible patients who wished to participate provided written informed consent, underwent a fasting blood draw, received dietary counseling on implementing the NCEP Therapeutic Lifestyle Changes diet, and initiated either a 4- or 6-week lead-in period depending on whether either a washout of a non-statin lipid-lowering therapy or an adjustment to the background statin was necessary.
Patients who did not require washout of non-statin lipid-lowering therapy: The screening visit occurred at Visit 1 (Week -6). Eligible patients entered a 4-week diet lead-in period and continued on their current dose of statin before the first TG/LDL-C qualifying visit (Visit 2/Week-2). Patients who required a change in their statin dose during the 2 weeks following Visit 1 entered a statin stabilization period so that the statin dose was stable for at least 4 weeks before the first TG/LDL-C qualifying visit (Visit 2/Week -2). At the discretion of the investigator, patients could be switched from a non-study statin to an allowed statin at Visit 1.
Patients who required washout of non-statin lipid-lowering therapy: The screening visit occurred at Visit 1 (Week -8). Eligible patients began a 6-week washout period before the first TG/LDLC qualifying visit (Visit 2/Week-2).
Qualifying period: At the end of either the 4-week or 6-week lead-in period, eligible patients had fasting LDL-C (calculated with Friedewald equation) and TG levels measured at Visit 2 (Week -2) and Visit 3 (Week -1).
The changes in lipid and lipoprotein parameters from baseline to Week 12 in the mineral oil placebo group are rather atypical for a trial that included a stabilization period for diet and lipid-lowering therapy, raising the possibility that mineral oil may not be as inert as assumed. If true, the treatment effects observed with AMR101 [Vascepa] may be overestimated.
Compared to placebo, LDL-C increased by 3.5% in the COMBOS trial using Lovaza, and decreased by 6.2% in the ANCHOR study using Vascepa 4 g/d. Compared to baseline, however, there were no differences in LDL-C in either trial. In other words, the difference in LDL-C response between Lovaza and Vascepa is due to the different LDL-C responses to placebo. In the Lovaza studies, lipids in the placebo arms were either unaffected by treatment or decreased to a small extent, whereas in the Vascepa studies, lipids increased more than would be expected (e.g. 9% increase in LDL-C and 6% increase in TGs in the placebo arm of the ANCHOR trial). The reason for the differences in placebo responses in unknown. It is possible that the Vascepa study populations became less adherent to lifestyle and/or pharmacologic therapy over the course of the trial. However, the elevation of atherogenic lipids in the placebo arms of the Vascepa trials raises the question of whether the light paraffin oil could have interfered with effectiveness of concomitant therapies.
…in ANCHOR, apoB increased 4 mg/dL on the 2 g/d dose [comprised of 2 g/d EPA + 2 g/d MO], decreased 3 mg/dL on the 4 g/d dose, and increased 7 mg/dL on the placebo. As noted previously, the reason for the consistent and substantial increase in apoB while on placebo is not apparent. Thus, one can conclude that either Vascepa (EPA-only) has apoB lowering effects not seen with EPA + DHA, or more likely, the placebo in these trials (light paraffin oil) was not wholly inert.
Reviewer Comment: Although the Vascepa 2g dose reduced TG, there were wide fluctuations in TG levels. By Week 11, the slight improvements in TG levels achieved at Week 4 were reduced back to almost the Baseline TG. Within one week (from Week 11 to Week 12) the mean percent change in TG changed from 0.20% to -9.78%. Wide fluctuations in TG were also observed in the Placebo group.
The Vascepa 4g dose reached maximum effectiveness by Week 4 and despite a slight decrease at Week 11 and Week 12, showed none of the wide fluctuations seen in Vascepa 2g or Placebo.
A meta-analysis of 32,258 patients of dyslipidemia was done by Philip J. Barter et al. It included 37 randomized studies of different types of statin (Rosuvastatin, atorvastatin, and simvastatin, etc.). Effect of these statins on HDL cholesterol level was assessed in this meta-analysis. They found that increase in serum HDL cholesterol was inversely related to dose of atorvastatin. There was 4.5% increase in serum HDL cholesterol with 10 mg dose while there was a 2.3% increase in serum HDL cholesterol with 80 mg dose of atorvastatin. It was concordant with our study which showed percentage increase in HDL-Cholesterol in the range of 9.52 ± 30.07 and 11.36 ± 28.62 at 3 and 6 months follow-up respectively in 40 mg group. While in 80 mg group, percentage increase in HDL-Cholesterol was 7.74 ± 26.43 and 9.02 ± 27.47 at 3 and 6 months follow-up respectively.
Compared to placebo in ANCHOR, IPE 4 g/day significantly decreased hsCRP levels in patients receiving higher (-29 %, p < 0.05) and medium (-23 %, p < 0.01) but not lower-efficacy statin regimens (+4 %, p > 0.05).
In ANCHOR, the changes from baseline in hsCRP for IPE 4 g/day and placebo in patients treated with atorvastatin were -12 and +31 %, respectively, resulting in a statistically significant placebo-adjusted reduction of 37 % (p = 0.0475). The changes from baseline in hsCRP for IPE 4 g/day and placebo in patients treated with rosuvastatin were -1.2 % and +15.2 %, respectively, resulting in a statistically significant placebo-adjusted reduction of 31 % (p = 0.0217). The changes from baseline in hsCRP for IPE 4 g/day and placebo in patients treated with simvastatin were 0.0 and +13.2 % respectively, resulting in a statistically non-significant placebo-adjusted reduction of 13.6 % (p = 0.0755).[15]
Amarin’s Complaint: In August 2017, Amarin filed a complaint with the Commission alleging that certain competitors are falsely labeling or deceptively describing synthetically produced omega-3 products as (or for use in) “dietary supplements” when the products are in fact “drugs” that have not been approved for sale or use in the United States. Appx19–29. (Amarin’s complaint applied only to a small group of synthetically modified products, not to the majority of fish oil dietary supplements.) Amarin alleged that those acts constitute unfair acts or unfair methods of competition under Section 337 of the Tariff Act. Appx24 ¶ 1; see 19 U.S.C. § 1337. Amarin also asserted that those unfair acts violate Section 43(A) of the Lanham Act because falsely labeling or deceptively describing drugs as (or for use in) dietary supplements deceives consumers and others in the supply chain regarding the nature of the product. Appx24 ¶ 1; see 15 U.S.C. § 1125(A)(1). Amarin alleged that its domestic-industry commercial interests were being injured as a result of certain competitors’ false and deceptive representations concerning the nature and characteristics of their imported products. Appx115–126.
As defined in section 201(FF)(1) of the FD&C Act (21 U.S.C. 321(FF)(1)), a “dietary ingredient” is any one of the following:
(A) A vitamin;
(B) A mineral;
(C) An herb or other botanical;
(D) An amino acid;
(E) A dietary substance for use by man to supplement the diet by increasing the total dietary intake; or
(F) A concentrate, metabolite, constituent, extract, or combination of any ingredient described in (A), (B), (C), (D), or (E).
5. If I alter the chemical structure of a dietary ingredient, is the new substance still a dietary ingredient?
It depends. Altering the chemical structure of a dietary ingredient (e.g., creation of new stereoisomers, addition of new chemical groups as in esterification) creates a new substance that is different from the original dietary ingredient. The new substance is not considered to be a dietary ingredient merely because it has been altered from a substance that is a dietary ingredient and, therefore, is in some way related to the dietary ingredient.
In some cases, however, the new substance may independently qualify for one of the dietary ingredient categories listed in section 201(FF)(1) of the FD&C Act. For example, taurine is the end product of the metabolism of the amino acid cysteine. It is thus a metabolite of an amino acid and fits one of the definitions of a dietary ingredient (see 21 U.S.C. 321(FF)(1)(D), (F)). The enzymatic or synthetic processing of cysteine or any other dietary ingredient would be an appropriate method for the manufacture of a metabolite of a dietary ingredient like taurine for use in a dietary supplement...
Based on the information in your submission, it is unclear if "fatty acid esters, derived from anchovy or menhaden oil" which you intend to market under the trade name Provinal™ is a "dietary ingredient" within the meaning of21 U.S.C. 32l(FF)(L). For example, synthetic fish oil fatty acid ethyl esters do not fit within the statutory definition of "dietary ingredient" because they are not constituents of a dietary substance for use by man under section 201(FF) (L)(F). Therefore, FDA cannot determine, at this time, whether your product contains a dietary ingredient that may lawfully be marketed as a dietary supplement.
If reagents used during processing are likely to make covalent changes to components in the mixture during processing, you should determine whether the new material is still a dietary ingredient. For example, use of a large amount of an oxidizing acid like sulfuric acid to process a botanical mixture may create a new “semi-synthetic” mixture that is no longer a mixture of components that were present in the original plant. Therefore, the mixture would no longer be a dietary ingredient.
DHA and EPA supplements can be given as free fatty acids, natural and reconstituted triglycerides and ethyl esters. Natural fish oil triglycerides (NTG) correspond to 100% triglycerides whereas chemically reconstituted triglycerides (RTG), as defined in the European Pharmacopeia are a mixture of monoglyceride (MG),12 diglyceride (DG) and triglycerides with triglyceride being the main component (>60%).
Until recently, Nordic Naturals ?sh oil products contained up to 60% triglycerides (with the remaining 40% comprised of diglycerides and monoglycerides). Now, however, we have perfected the technology that allows us to reassemble 93% of the fatty acids in our ?sh oils into the triglyceride form (with only 7% monoglycerides and diglycerides).
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A metabolite that has been synthesized from another dietary ingredient would be a dietary ingredient under section 201(FF)(1)(F) and could be used as a dietary ingredient in a dietary supplement. Although the definition of a metabolite requires human ingestion of the dietary ingredient to increase the production or flux of the metabolite in the human body, it does not require the metabolism to actually take place in a human being during the manufacture of a dietary ingredient. A metabolite may be synthetically produced, provided that the starting material is a dietary ingredient and the production process mimics the metabolic process in the body following ingestion.
FDA can create an exception to this prohibition by regulation, but only if the agency finds that the use of the article in dietary supplements would be lawful. To date, no such regulations have been issued. The appropriate mechanism to request such a regulation is to file a citizen petition under 21 CFR 10.30.
Practically and scientifically, pure ethyl alcohol synthesized from natural gas or petroleum products does not differ from that obtained by fermentation with subsequent distillation. Furthermore, foods in which one is used cannot be distinguished objectively from those in which the other is used.
POLICY:
Synthetic ethyl alcohol may be used as a food ingredient or in the manufacturing of vinegar or other chemicals for food use, within limitations imposed by the Federal Food, Drug, and Cosmetic Act, the Alcohol Administration Act, and regulations promulgated under these acts.
A number of intracellular proteins have been isolated from different sources and shown to catalyze esterification of fatty acids to ethanol (12–14). By aminoterminal-sequence analysis, it was shown that two of these purified FAEE synthases are apparently identical to liver microsomal carboxylesterase ES-10, the predominant carboxylesterase in rat liver (15, 16). Other enzymes such as pancreatic cholesterol ester synthase (17) and pancreatic carboxylester synthase (18) also have been shown to possess some FAEE synthesizing activity. FAEE also can be synthesized by transesterification of ethanol and fatty acyl-CoA, a reaction catalyzed by acylcoenzyme A:ethanol O-acyltransferase (AEAT).
Synthetic vitamins, minerals, and amino acids are recognized as dietary ingredients because a vitamin, mineral, or amino acid is defined by its nutritional function (its ability to provide nutrients to the human body), not by its state of matter like a botanical.
FDA respectfully submits that the Commission should decline to initiate the requested investigation. As pled, Complainants’ claims—unfair methods of competition under the Tariff Act based on false advertising under the Lanham Act and violations of the Federal Food Drug and Cosmetics Act (“FDCA”)—can succeed only if the Commission finds that Respondents’ products are unapproved “new drugs” rather than “dietary supplements” under the FDCA. The Complaint here is predicated on open questions of law and policy on which FDA has not reached final conclusions. Any such findings by the Commission on those issues may conflict with later determinations by FDA. Further, through the Complaint, Complainants attempt an unlawful private FDCA enforcement action based on Complainants’ allegations, not on FDA’s findings. As detailed below, because Congress has authorized only FDA to initiate FDCA enforcement actions, the FDCA precludes claims that would require the adjudicator to interpret, apply, or enforce the FDCA. For Complainants to succeed on any of their claims, the Commission would have to do all three of those things.
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