Materials and MethodThe present stu

Materials and Method
The present study was carried out in the Biotechnology Laboratory of the Bangladesh Agricultural Research Institute (BARI), Joydebpur, Gazipur-1701, Bangladesh during the period from September 2004 to June 2005. The planting materials of BARI Banana-I were collected from Biotechnology Division, BARI, Joydebpur, Gazipur. The meristem was obtained from developing suckers of about four months of age grown under field conditions and was brought to the preparation room. The suckers were washed thoroughly under running tap water. The roots and outer tissues of the suckers were removed with the help of a sharp knife. A number of outer leaves were removed until the shoot measured about 1.0-2.0 cm in length and 1.0 cm width at the base. The meristem used for establishment of culture was prepared through dissection and removal of leaf sheath under the microscope. Then the initial explant was prepared under stereomicroscope by removal of outer tissue of meristem with the help of sterile scalpel, which was about 5x5 mm in size.
Two experiments were conducted to assess the effect of different concentrations of BAP, NAA, IAA and IBA on shoot proliferation and subsequent rooting of the multiplied shoot. In the frist experiment, in vitroderived banana cv. BARI Banana-I plantlets were used as sources of meristem to investigate the effect of BAP, NAA each at different concentrations alone or in combinations on shoot proliferation. Five levels of BAP (0.0, 2.5, 5.0, 7.5, and 10.0 mg/l) and 5 levels of NAA (0.0, 0.5, 1.0, 1.5 and 2.0 mg/l were used. All the combinations of both BAP and NAA were used as treatments. In the second experiment, there were 3 levels of IAA (0.0, 0.5 and 1.0 mg/l) and 4 levels of IBA (0.0, 0.5, 1.0, and 1.5 mg/l) were used as treatments. The experiments were arranged in completely randomized design (CRD) with 4 replications. Each treatment consisted of 10 culture tubes per replication. Data were collected on the effect of different treatments on shoot proliferation and rooting.
Murashige and Skoog (1962) medium supplemented with different phytohormones as per treatments were used as culture medium for shoot induction, shoot multiplication and maintenance and regeneration of roots from multiplied shoot. Hormones were added separately to different media according to the requirements. For the preparation of media, stock solutions were prepared at the beginning and stored at 9±1°C temperature. The respective medium was prepared from the stock solutions. The culture tubes with media were then autoclaved at 1.06 kg/cm2 pressure at 121°C for 25 minutes. The medium was then cooled at room temperature before use.
The pale white tissue block (l.0 × 2.0 cm) containing meristem and rhizomatous base were taken in a beaker. Surface sterilization was done under laminar Airflow Cabinet with 70% ethyl alcohol, the explants were surface sterilized with 0.1% mercuric chloride and a few drops of Tween 20 for 15 minutes. Finally, the explants were then rinsed three to four times with steriledistilled water.
The isolated and surface sterilized explants were collected carefully under the stereomicroscope through maintaining aseptic condition inside the laminar air flow cabinet to use those as explants. The individual meristems were directly inoculated to each of the culture tube containing 20 ml of MS medium supplemented with different concentrations of hormones as per treatment covered with aluminium foil.
The culture tubes were transferred to growth room and allowed to grow in controlled environment. The temperature of the growth room was maintained within 25±1°C by an air conditioner. A 16-hour light period was maintained with light intensity of 2000 lux for the growth and development of culture.
Some explants become black in colour within 6-7 days after inoculation. To control blackening after about one week, the blackish tissues on the explants were removed and the meristematic tissues were, transferred to similar fresh medium. It was repeated 10 days interval for about one month to minimize further blackening of the tissues.sub-culturing, the entire samples of in vitro shoot were cut into small pieces so that each piece would contain about one shoot. Leaf and blackish or brownish basal tissues were removed to expose the meristems. Each piece was inoculated into a similar fresh medium. It was practiced at the interval of every one month.
When the shoots grew about 3-5 cm in length with 3-6 well developed leaves, they were rescued aseptically from the culture tubes and were separated from each other and again cultured on freshly prepared medium containing different combinations of hormonal supplements for root induction.
Potting mixture containing ground soil and cowdung in the ratio of 1:1 was mixed thoroughly and were placed into a 10 × 15 cm polythene bag for growing in vitro grown plantlets under ex vitro conditions.