ASD-STAN PREN 4159-2005 Aerospace series Paints and varnishes Determination of resistance to microbial growth (Edition P 1)《航空航天系列 油漆和清漆 微生物生长抑制性测定 第P1版》.pdf
《ASD-STAN PREN 4159-2005 Aerospace series Paints and varnishes Determination of resistance to microbial growth (Edition P 1)《航空航天系列 油漆和清漆 微生物生长抑制性测定 第P1版》.pdf》由会员分享,可在线阅读,更多相关《ASD-STAN PREN 4159-2005 Aerospace series Paints and varnishes Determination of resistance to microbial growth (Edition P 1)《航空航天系列 油漆和清漆 微生物生长抑制性测定 第P1版》.pdf(8页珍藏版)》请在麦多课文档分享上搜索。
1、ASD STANDARD NORME ASD ASD NORM prEN 4159 Edition P1 November 2005 PUBLISHED BY THE AEROSPACE AND DEFENSE INDUSTRIES ASSOCIATION OF EUROPE - STANDARDIZATIONGulledelle 94 - B-1200 Brussels - Tel. + 32 2 775 8126 - Fax. + 32 2 763 3565 - www.asd-stan.orgICS: Descriptors: ENGLISH VERSION Aerospace seri
2、es Paints and varnishes Determination of resistance to microbial growth Srie arospatiale Peintures et vernis Dtermination de la rsistance laction des microorganismes Luft- und Raumfahrt Anstrichstoffe Bestimmung der Widerstandsfhigkeit gegen Schimmelwachstum This “Aerospace Series“ Prestandard has b
3、een drawn up under the responsibility of ASD-STAN (The Aerospace and Defense Industries Association of Europe - Standardization). It is published for the needs of the European Aerospace Industry. It has been technically approved by the experts of the concerned Domain following member comments. Subse
4、quent to the publication of this Prestandard, the technical content shall not be changed to an extent that interchangeability is affected, physically or functionally, without re-identification of the standard. After examination and review by users and formal agreement of ASD-STAN, it will be submitt
5、ed as a draft European Standard (prEN) to CEN (European Committee for Standardization) for formal vote and transformation to full European Standard (EN). The CEN national members have then to implement the EN at national level by giving the EN the status of a national standard and by withdrawing any
6、 national standards conflicting with the EN. Edition approved for publication 30 November 2005 Comments should be sent within six months after the date of publication to ASD-STAN Non-metallic Material Domain Copyright 2005 by ASD-STAN prEN 4159:2005 2 Contents Page Foreword2 Introduction.3 1 Scope 3
7、 2 Terms, definitions and abbreviations3 3 Principle3 4 Apparatus .4 5 Specimen4 6 Procedure .5 6.1 Test methods5 6.1.1 Preparation of agarose + glucose gel5 6.1.2 Application of gel to coating 5 6.1.3 Preparation of spore suspension.5 6.1.4 Application of suspension to gel and storage at 25 C .5 6.
8、1.5 Microscopic examination5 6.1.6 Time course of germination6 7 Designation 7 8 Test report 7 Bibliography8 Foreword This standard was reviewed by the Domain Technical Coordinator of ASD-STANs Non-metallic Material Domain. After inquiries and votes carried out in accordance with the rules of ASD-ST
9、AN defined in ASD-STANs General Process Manual, this standard has received approval for Publication. prEN 4159:2005 3 Introduction Certain fungi are known to be capable of proliferating in fuel systems which can cause corrosion and blockage. Conidiospores are the dispersal form of these fungi. Germi
10、nation of conidia is the first stage in proliferation of the fungus. If the conidiospore cannot germinate, there can be no proliferation and no blockage of fuel lines, ducts etc. This method should be performed only by persons qualified in the microbiology of fungi. The standard can be used to asses
11、s the effectiveness of new candidate coating systems in inhibiting microbial (fungal) growth. 1 Scope This standard specifies a method to assess the ability of biocide-containing coatings to prevent the germination of conidiospores of certain fungi known to be capable of proliferating in fuel system
12、s for aerospace applications. 2 Terms, definitions and abbreviations For the purposes of this standard, the following terms, definitions and abbreviations apply. Conidiospores are typically single-celled structures produced by the mycelial mould form of the fungus. Conidiospores are spherical or nea
13、rly spherical resting cells, i.e. cells which may be dispersed readily but which do not proliferate. However, conidiospores may germinate if they encounter suitable conditions of moisture and nutrients. On germination, a conidiospore produces a long tube-like outgrowth which then forms dense branchi
14、ng structures mycelia which may block fuel ducts etc. A suitable coating will prevent germination of conidiospores. A coating which prevents germination of conidiospores is considered to have fungistatic activity. This fungistatic activity may be assessed quantitatively by assessing the success rate
15、 of germination of conidiospores under standard conditions (see below) to determine whether the test coating delays or prevents germination of conidiospores when compared with a coating which is known to possess no fungistatic activity. Laboratories which undertake work to this method should first o
16、btain the test fungi (see 5) and perform control experiments to satisfy themselves that they can follow the process of germination of conidiospores. These initial experiments may be performed by placing the agarose gel (see below) on the surface of sterile plastic petri dishes rather than on the sur
17、face of coated test panels, as is done in the present method. 3 Principle 3.1 Conidiospores are placed on a gel within a few millimetres of the panel/coating under test. Under the test conditions a high proportion of these conidia germinate begin growth rapidly unless some material in the coating di
18、ffuses through the gel and prevents germination. 3.2 The success rate of germination, after any given interval of exposure to the coating, is expressed as the number of cells that have germinated divided by the number of cells examined (germinated + nongerminated). The success rate of germination is
19、 determined from time to time, beginning when the conidiospores are first exposed to the coating under test. Examination is made using a microscope 100. This allows ready distinction between ungerminated conidiospores approximately spherical and the long filamentous outgrowth that is the result of g
20、ermination. prEN 4159:20054 3.3 The results obtained with conidiospores exposed to test coatings are to be compared with results of conidiospores exposed to coatings that contain no inhibitor. 4 Apparatus 4.1 Incubator, capable of maintaining (25 1) C. 4.2 Autoclave suitable for sterilization of mic
21、robiological growth media, i.e. capable of heating the media to 121 C for 15 minutes. 4.3 Water bath, set to (45 1) C. 4.4 Microscope, magnification 100, and glass microscope slides. 4.5 Plastic disposable petri dishes : 90 mm to 100 mm diameter. 4.6 Sterile microbiological loops. Commercially avail
22、able disposable plastic loops (stated to carry 10 microlitres) are suitable. 4.7 Haemocytometer (blood cell counting chamber) Neubauer ruling. 4.8 Funnel, loosely plugged with nonabsorbent cotton wool. 4.9 Balance, toploading, 0,1 g resolution. 4.10 Micropipetting device (with disposable sterile tip
23、s) to deliver 0,010 ml. 4.11 Test fungi, to be obtained from national culture collections: 4.11.1 Amorphotheca resinae (also known as Cladosporium resinae) 4.11.2 Aspergillus niger 4.11.3 National culture collections contain several different strains of each of these fungi. The laboratory should cho
24、ose a suitable strain (e.g. one isolated from aeronautical fuel tank) by reference to the information supplied by the culture collection. 4.12 Microbiological growth media Rose Bengal Chloramphenicol Agar. The Oxoid product Rose Bengal Chloramphenicol Agar is suitable. 4.13 Agarose The product catal
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