Laboratory and Growth Room Conditions. Sterile (aseptic) technique/environment Aseptic technique is absolutely necessary for the successful establishment.

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Presentation transcript:

Laboratory and Growth Room Conditions

Sterile (aseptic) technique/environment Aseptic technique is absolutely necessary for the successful establishment and maintenance of plant cell, tissue and organ cultures. Why? The in vitro environment in which the plant material is grown is also ideal for the proliferation of microorganisms. In most cases the microorganisms outgrow the plant tissues, resulting in their death.

Sterile (aseptic) technique/environment Contamination can also spread from culture to culture. The purpose of aseptic technique is minimize the possibility that microorganisms remain in or enter the cultures.

Sterile (aseptic) technique/environment The environmental control of air is also of concern because room air may be highly contaminated. Example: Sneezing produces 100, ,000 droplets which contain a lot of microorganisms. These contaminated particles may be present in the air for weeks. Air may also contain bacterial and fungal spores, as do we.

Contamination

Contaminants – Bacteria Bacteria are the most frequent contaminants. They are usually introduced with the explant and may survive surface sterilization of the explant because they are in the interior tissues.

Contaminants – Bacteria

Some bacterial spores can also survive the sterilization procedure even if they are on the tissue surface. Bacteria can be recognized by a characteristic “ooze“. The ooze can be many colors including white, cream, pink, and yellow. There is also often a distinctive odor.

Contaminants – Fungi Fungi may enter cultures on explants or spores may be airborne. Fungi are frequently present as plant pathogens and in soil. They may be recognized by their “fuzzy” appearance, and occur in different colors.

Contaminants – Fungi

Contaminants – Virus Viruses are extremely small organisms that are not easily detected. Thus, plant culture is not necessarily pathogen-free even if microorganisms are not detected, and this can influence culture success. Special measures such as meristem culture are often necessary to eradicate such contaminants.

Initial contaminants Most contamination is introduced with the explant because of inadequate sterilization or just very dirty material. Initial contamination is obvious within a few days after cultures are initiated.

Latent contamination Contamination that is observed long after cultures are initiated is usually bacterial. Apparently the bacteria are present endogenously in the initial plant material and are not obviously pathogenic in situ. Latent contamination is particularly dangerous because it can easily be unknowingly transferred among cultures.

Introduced contamination Contamination can also occur as a result of poor sterile technique or dirty lab conditions. This kind of contamination is largely preventable with proper care.