JP2008120722A - Placebo for use with biologic - Google Patents

Abstract

<P>PROBLEM TO BE SOLVED: To provide a placebo which is substantially identical with a biologic in appearance, is pharmaceutically safe, has no efficacy unlike a biologic, and is capable of being handled in the same manner as in an investigational new drug used in e.g., a double blind method. <P>SOLUTION: The placebo for use with a biologic contains a substance having surface activity. Desirably, the placebo is one wherein the substance having surface activity is a surfactant. <P>COPYRIGHT: (C)2008,JPO&INPIT

Description

  The present invention relates to a placebo for a biological product used in clinical trials.

  The double-blind method, which is one of the clinically correct methods for evaluating the drug effect, is carried out particularly to avoid psychological effects. That is, only the third grader who knows the distinction does not inform both the patient and the doctor of the distinction between the test drug and the placebo. Therefore, it is essential that the test drug and placebo are indistinguishable in terms of appearance, taste, smell, and the like.

  At present, for example, physiological saline is used as an alternative to placebo for globulin preparations and the like, but plasma fractionation preparations have a foamy appearance, so physiological saline with a different appearance is placebo. As was not appropriate. That is, during clinical trials, in order to ensure blindness, the preparation and dilution of the preparation are performed in a separate room, and the preparation container is covered with a complicated procedure such as covering. In addition, it is necessary to separate the doser and the effect-determiner from the drug preparer. In some cases, an albumin-containing placebo is used as a placebo for globulin preparations, but it is similar in appearance but may be colored, and it cannot be said to be a suitable placebo in terms of efficacy and safety.

  However, there is no known placebo for biological products that are safe and have the same conditions as placebo without any difference in appearance.

  An object of the present invention is to provide a placebo that has almost the same appearance as a biological product and is pharmaceutically safe but has no medicinal effect and can be handled in the same manner as a test drug in a double-blind method or the like. That is.

As a result of repeated studies on the solution of the above problems, the present inventors have found that a composition containing a surface active substance has the same appearance as a biological product, and has a safe and stable quality. It was found that it can be used as a placebo, and the present invention has been completed.
That is, the present invention is as follows.
(1) A placebo for a biological product containing a substance having a surface active action.
(2) The placebo according to (1), wherein the substance having a surface active action is a surfactant.
(3) The placebo according to (2), wherein the surfactant content is 0.00001 to 0.010 w / w%.
(4) The placebo according to (1), wherein the substance having a surface active action is a polysaccharide.
(5) The placebo according to (4), wherein the polysaccharide content is 20 to 0.1 w / v%.
(6) The placebo according to any one of (1) to (5), wherein the biological product is a plasma fractionation preparation.
(7) The placebo according to (6), wherein the plasma fractionated preparation is a globulin or albumin preparation.
(8) The placebo according to any one of (1) to (7), further comprising an isotonic agent.
(9) A double-blind method using a placebo of a biological product containing a substance having a surface active action.
(10) The double-blind method according to (9), wherein the substance having a surfactant action is a surfactant.
(11) The double-blind method according to (9), wherein the substance having a surfactant activity is a polysaccharide.

  According to the placebo of the present invention, in clinical trials, it is indistinguishable from the test drug in appearance and can be treated in the same way as the test drug, so the reliability of the test when used in clinical trials, particularly double-blind methods Will improve.

The placebo of the biological product in the present invention refers to a product having substantially the same appearance as the product and containing no active ingredient. Examples of biological products that are subject to placebo in the present invention include plasma fractionated preparations, vaccine preparations, toxin preparations, toxoid preparations, antitoxin preparations, leptospiral serum preparations, blood preparations, recombinant protein preparations, cultured cell-derived protein preparations, Examples include monoclonal antibody protein preparations, heparin preparations, and the like.
Preferred are plasma fractionated preparations, vaccine preparations, recombinant protein preparations, cultured cell-derived protein preparations, monoclonal antibody protein preparations, heparin preparations, and the like.

  Examples of the plasma fraction preparation in the present invention include albumin preparation, immunoglobulin preparation, coagulation factor preparation, antithrombin-III preparation, fibrinogen preparation, thrombin preparation and the like. Preferred are immunoglobulin preparations, antithrombin-III preparations, coagulation factor preparations and fibrinogen preparations, and more preferred are immunoglobulin preparations.

  The placebo of the present invention is not particularly limited as long as it is indistinguishable from a biological product that is a test drug in appearance. Moreover, the test drug used as a control for the placebo of the present invention may be liquid or powder. Therefore, any placebo of the present invention may be selected according to the mode of the test drug. In particular, when the test drug is a liquid preparation, the liquid placebo is suitable for the double-blind method because the clinical trial can be performed without distinction even during preparation and dilution.

  The placebo of the present invention contains a substance having a surface active action in order to have foamability equivalent to that of a biological product when it becomes liquid. The surface active action refers to an action of reducing interfacial tension by strongly adsorbing a substance dissolved in one or two phases at the interface when two phases are in contact with each other. In the present invention, this particularly means a case where a substance dissolved in the liquid acts on the gas-liquid interface. A substance having a surface-active action has a portion having a contradictory property of a hydrophobic group and a hydrophilic group in its molecule, and is sometimes called an amphiphilic substance. Substances that exhibit significant surface activity even in small amounts are referred to as surfactants.

  Examples of the substance having a surface active action include surfactants and polysaccharides. In the present invention, the surfactant and the polysaccharide may be used in combination, and are not particularly limited as long as they are pharmaceutically acceptable.

  Surfactants include sorbitan sesquioleate, sorbitan fatty acid ester, polyoxyethylene sulfide castor oil 60, polyoxyethylene sorbitan monolaurate, polyoxyethylene (160) polyoxypropylene (30) glycol, polysorbate 20, polysorbate 80 And macrogol 400, and the like, preferably polysorbate 20, polysorbate 80, and macrogol 400, and more preferably polysorbate 20 and polysorbate 80. These surfactants may be used alone or in combination of two or more. The polysaccharide is preferably dextran 40.

The surfactant in the present invention is usually contained at 0.00001 to 0.010 w / v%, preferably 0.00001 to 0.004 w / v%, based on the total amount of placebo.
The polysaccharide in the present invention is usually contained in an amount of 20 to 0.1 w / v%, preferably 10 to 1 w / v%, based on the total amount of placebo.

  The placebo of the present invention desirably contains an isotonic agent in order to achieve an osmotic pressure equivalent to that of a biological product. The isotonic agent is not particularly limited as long as it is pharmaceutically acceptable. The tonicity agent may be the same as or different from the test drug. Isotonic agents include amino acids such as glycine, sugar alcohols such as D-sorbitol and D-mannitol, sugars such as lactose, maltose, and glucose, and sodium chloride (saline), sodium bicarbonate, citric acid. Sodium phosphate, sodium hydroxide, sodium lactate, phosphoric acid, sodium hydrogen phosphate, potassium dihydrogen phosphate, sodium dihydrogen phosphate, etc., preferably D-sorbitol, glycine, sodium chloride, sodium bicarbonate, citric acid Examples thereof include sodium acid, D-mannitol, lactose, sodium hydroxide, sodium chloride (saline solution), glucose, sodium lactate, phosphoric acid, sodium hydrogen phosphate, potassium dihydrogen phosphate, sodium dihydrogen phosphate and the like. These tonicity agents may be used alone or in combination of two or more.

  The concentration of the isotonic agent in the present invention can be appropriately adjusted to an osmotic pressure capable of being intravenously injected. Generally, intravenous injection is possible within an osmotic pressure ratio range of 0.25 to 4. The concentration of the tonicity agent is, for example, 1 to 20 w / v% (preferably 2 to 10 w / v%) sorbitol.

  The placebo of the present invention may contain a pH buffer. The pH buffer is not particularly limited as long as it is pharmaceutically acceptable. As pH buffering agent, sodium hydroxide, hydrochloric acid, phosphoric acid, sodium hydrogen phosphate, potassium dihydrogen phosphate, sodium dihydrogen phosphate, citric acid, sodium citrate, disodium citrate, glycine, sodium L-glutamate , Acetic acid, sodium acetate, lactic acid, sodium lactate, anhydrous citric acid, anhydrous sodium citrate, anhydrous sodium acetate and the like, preferably phosphoric acid, sodium hydrogen phosphate, potassium dihydrogen phosphate, sodium dihydrogen phosphate, Examples include citric acid, sodium citrate, disodium citrate, glycine, sodium L-glutamate, acetic acid, sodium acetate, lactic acid, sodium lactate, and anhydrous citric acid. You may use these pH buffer agents individually or in combination of 2 or more types.

  The placebo of the present invention is preferably adjusted to the pH of the control drug by adding a pH buffer. Generally, a neutral pH is a preferable pH range for a preparation that can be intravenously injected. In the present invention, the preferred pH range is pH = 3 to 7.5, more preferably pH = 3.5 to 6.0.

  The placebo of the present invention includes pharmacologically acceptable stabilizers, dispersants, preservatives, solubilizers, solubilizers, soothing agents, coloring agents, and the like, which are generally used in pharmaceuticals within the scope of the present invention. An additive such as an agent can be appropriately blended. These additives are usually blended in the proportions used for pharmaceuticals.

  The placebo administration method of the present invention is not particularly limited as long as it is the same administration method as the test drug, such as intravenous injection or intramuscular injection. The dose, the number of administrations per day, the administration period, etc. are not particularly limited as long as they are the same as the test drug. For example, the daily dose can be calculated based on the body weight of the subject, and the administration rate can be administered with attention to the precautions described in the package insert.

The placebo of the present invention can be produced, for example, as follows.
A necessary amount of a substance having a surface-active effect is added to water for injection and stirred. If necessary, an appropriate amount of isotonic agent or pH buffering agent is added and stirred, and the osmotic pressure or pH is confirmed. The obtained solution is subjected to a sterilization process. A preferred embodiment of the sterilization step is filter filtration. After the sterilized solution is dispensed and wound, it can be subjected to a sterilization step if necessary. A preferable method for the sterilization step is high-pressure steam sterilization.

  The placebos of the present invention may be used according to “standards for conducting clinical trials of pharmaceuticals”. Conventionally, when physiological saline is used as a placebo, it cannot be administered in the same procedure as the test drug because the appearance is different from the test drug as described above. Therefore, the clinical trial implementation plan states that, for example, “preparation and dilution are performed without touching the eyes of the prescriber and effector during the clinical trial, and the physiological saline container is covered”. Therefore, it was necessary to describe a specific method for maintaining blindness. However, in a clinical trial using a placebo in the present invention, the test can be carried out in the same manner as the test drug, so it is only necessary to describe the placebo name in the name of the control drug in the study protocol. There is no need to perform complicated procedures to ensure blindness. Therefore, the test can be easily performed by using the placebo of the present invention, and the reliability of the clinical test (especially in the double blind test) is improved.

  The present invention also provides a double-blind method using a placebo of a biological product containing a substance having a surface-active effect, the method comprising the step of administering the placebo in exactly the same procedure as the test drug.

  EXAMPLES Hereinafter, although an Example demonstrates this invention in detail, this invention is not limited to these at all.

(Example 1) Preparation of placebo for immunoglobulin preparation A solution obtained by adding 10.53 g of Na ₂ HPO ₄ · 12H ₂ O (Kanto Chemical) to 20 L of water for injection at room temperature and NaH ₂ PO ₄ · 2H in 12 L of water for injection at room temperature _The solution to which 8.29 g of ₂ O (Kishida Chemical) was added was mixed. After confirming that the pH of the mixed solution was 6.5 to 7.5, 1600 g of sorbitol (Nikken Chemical) was added. This solution is designated as Solution 1.
1 L was collected from the solution 1, and 2 g of polysorbate 80 (Tween 80) (Sanyo Chemical Industries) was added and stirred. This solution is designated as Solution 2.
In a cold place, they were mixed at a ratio of Solution 1: Solution 2 = 99: 1 (volume ratio) and stirred. This solution was sterilized by filtration through a 0.22 μm filter (Nippon Millipore). Thereafter, 50 mL each was dispensed, stoppered and wound, and a placebo was prepared (Table 1).

(Example 2) Storage stability test The placebo prepared in Example 1 was subjected to an acceleration test to examine storage stability.
The storage conditions were stored at 25 ° C., and the storage period was 6 months.
The test items were a property and indistinguishability test, a pH test, an insoluble foreign matter test, and an insoluble fine particle (n = 3).
As the immunoglobulin preparation to be tested, blood donated venoglobulin-IH _Yoshitomi (Benesis Co., Ltd.) was selected.

(1) Property and Indistinguishability Test Regarding the placebo and blood donation Venoglobulin-IH _Yoshitomi prepared in Example 1, 1. In accordance with the essence and properties, the properties were confirmed, and the test was performed by observing the appearance when mixed by 10 rotations at a speed of one reciprocation in about 2 seconds.

(2) pH test A test was conducted in accordance with the pH measurement method of the biologics standard.

(3) Insoluble foreign matter inspection The test was conducted by applying the Japanese Pharmacopoeia (14th revision), general test method, and insoluble foreign matter inspection method No. 1 of injections. The criterion of judgment is “no clear insoluble foreign matter that is clear and easily detected”.

(4) Insoluble fine particle test Japanese Pharmacopoeia (14th revision), General rules for pharmaceutical preparations, Insoluble fine particle test method No. 1 for injections and General test method Insoluble fine particle test method No. 1 are applied mutatis mutandis. It was.

(5) Equipment Used The main equipment used for the test is a pH meter (F-14, Horiba Seisakusho), an osmometer (OM-6030, Arkray), a fine particle measuring device (8000A type, HIAC / Royco) and the like.

(6) Results As shown in Table 2, the placebo prepared in Example 1 showed no change in appearance at 25 ° C. and 6 months, and was also indistinguishable from the test drug. Further, at 25 ° C. for 6 months, no large pH fluctuation was observed as shown in Table 3, and no insoluble foreign matter was generated and no increase in insoluble fine particles was observed. Therefore, the safety as a pharmaceutical was ensured.

Claims (11)

  A placebo of a biological product containing a substance having a surface active action.   The placebo according to claim 1, wherein the substance having a surfactant activity is a surfactant.   The placebo according to claim 2, wherein the content of the surfactant is 0.00001 to 0.010 w / w%.   The placebo according to claim 1, wherein the substance having a surface active action is a polysaccharide.   The placebo according to claim 4, wherein the content of the polysaccharide is 20 to 0.1 w / v%.   The placebo according to any one of claims 1 to 5, wherein the biological product is a plasma fractionation preparation.   7. The placebo according to claim 6, wherein the plasma fractionation preparation is a globulin or albumin preparation.   The placebo according to any one of claims 1 to 7, further comprising an isotonic agent.   A double-blind method using a placebo of a biological product containing a substance having a surface-active effect.   The double-blind method according to claim 9, wherein the substance having a surfactant activity is a surfactant.   The double-blind method according to claim 9, wherein the substance having a surfactant activity is a polysaccharide.