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in vitro culture and isoenzyme analysis of giardia lamblia

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dislodged by chill<strong>in</strong>g the <strong>culture</strong> tubes <strong>in</strong> an ice bath for 20 m<strong>in</strong>utes. Thereafter the<br />

tube contents were mixed by gentle <strong>in</strong>version <strong>and</strong> centrifuged at 400xg for 5m<strong>in</strong> at<br />

4°C. Old supernatant medium was gently decanted <strong>and</strong> pelletted trophozoites<br />

resuspended <strong>in</strong> 1 ml <strong>of</strong> fresh TYI-S-33. A 1: 10 dilution <strong>of</strong> trophozoites was<br />

prepared <strong>in</strong> 1 % formal<strong>in</strong> <strong>in</strong> a clean tube to fix <strong>and</strong> enumerate the trophozoites.<br />

Aliquots <strong>of</strong> 0,1 ml <strong>of</strong> the rema<strong>in</strong><strong>in</strong>g trophozoite suspensions conta<strong>in</strong><strong>in</strong>g 1 x1 0 4 cells<br />

fml were distributed to two or more tubes conta<strong>in</strong><strong>in</strong>g 7ml TYI-S-33 medium. The<br />

exp<strong>and</strong>ed <strong>culture</strong>s were ma<strong>in</strong>ta<strong>in</strong>ed as above until confluent monolayers were<br />

obta<strong>in</strong>ed for cryopreservation (Chapter 6) <strong>and</strong> preparation <strong>of</strong> Iysates for<br />

<strong>isoenzyme</strong> electrophoresis (Chapter 7).<br />

112

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