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MAINTENANCE OF LONG-TERM CULTURES

Some fungi require over six months to sporulate (such as sporocarpic species formerly in Sclerocystis). Others produce spores and other propagules which break-down rapidly in dry storage and therefore some or all of the germplasm must be maintained in long-term cultures. We use several procedures to avoid keeping the culture in the same pot for longer than five months. Why not just keep the culture growing as long as the host plant in the pot remains viable? There are several reasons:

1. Most root growth (at least for sorghum/sudangrass) occurs in the first three months of a pot culture. During the next month or two, when the plant is static, sporulation will increase dramatically (if sporulation is to occur at all -- see our interpretation of this phenomenon here). After that, both plants and their fungal inhabitants stagnate and often begin to deteriorate or senesce. This is especially true of plant roots, which can degrade amazingly fast depending on moisture/temperature conditions. Regardless of greenhouse cleanliness and other measures taken to reduce introduction of contaminants, saprophytes, commensals, and even some beneficial microbes will naturally colonize pot contents. We typically average 103 colony-forming units of bacteria, fungi, and actinomycetes in our pot cultures. After 5 months, these numbers will increase dramatically, probably because of an increase in organic residues in the pot culture medium. We observe visible declines in spore counts and infectivity measurements in cultures maintained in the same pot for 6-7 months or longer.

2. Even if there are no problems that arise during extended pot culture development, the increase in degraded organic matter in old pot cultures creates a new set of problems for long-term storage. In our experience, cultures grown for even five months cannot be stored as long as those grown for 3-4 months. We hypothesize that even with drying and refrigeration, microbial activity still occurs at some level that utilizes fungal propagules as substrate. It stands to reason that the higher the inoculum potential of these microbes, the more activity will occur with a concomitant acceleration of deterioration of fungal propagules in the inocula.

3. In addition to storage problems from repeated propagation cycles for an accession culture, we also are finding that newly formed spores more rapidly degrade or are parasitized while the culture is actively growing. At harvest, therefore, anywhere from 50-90% of the sporulation in the pot culture will consist of unhealthy or dead spores. Occurrence of this problem is becoming more prevalent as a significant number of accessions are in their16th to 17th successive propagation cycle after being in the collection for more than 15 years (see figure at right). To solve this problem, new cultures are started from extracted spores in any culture with more than 25% of spores degraded or parasitized. The extensive variation in number of propagation cycles before significant degradation occurs is due to differences in fungal susceptibility -- with most of the fungi in cycles 2-4 being either Gigaspora species or Glomus clarum.

Reseeding

A pot culture can be reseeded with a good chance of success as long as it has been growing for at least 30 days (post-emergence). Reseeding is done early in pot culture development usually when plant hosts are compromised in some way that also doesn't destroy fungal infectivity. Examples are plants irreversibly wilted due to interruption in watering or unfavorable temperatures or biological or physical variables caused premature death of plants (improper use of insecticides, etc.).

1. All work is done on a surface-sterilized table (e.g. alcohol swab) covered with 1-2 layers of newsprint.

2. Massage the pot to loosen contents from edges, and gently pull shoots to move contents (held together by roots and hyphae) slightly out of the pot.

3. We use flame surface-sterilized surgical scissors to cut all stems in a pot approximately one centimeter below the soil surface. Any sharp utensil, such as a scalpel, also can be used. By holding the shoots, there is a minimum amount of disturbance. Growth medium is gently shaken from around shoots, and the shoots are discarded.

4a. For young pot cultures (shown here) or cultures where propagule levels are determined to be extremely low or poorly infective (based on MIP, colonization levels, etc.), then pot contents should not be disturbed and seeds of the same host added to the cut surface. Cover seeds with left over soil or growth medium and water. Grow for another 4-5 months.

4b. If fungal propagule levels are higher and can tolerate some disturbance or dilution, then the pot contents can be cut into quarters. Two of these quarters are placed back in the pot and massaged to loosen root mats. Then add sterile growth medium and mix gently with the loosened quarters (so they aren't broken up very much). Add seed, cover with sterile media, and water. Grow for another 4-5 months.

5. Repeat steps 1-4 for additional propagation cycles, if necessary. The most important considerations are: (i) leave a portion of the parent pot culture contents relatively undisturbed to maintain hyphal networks and spore-hyphal aggregates, (ii) use half or less of pot culture contents to start the next cycle if propagule levels are high enough to be diluted (thus reducing buildup of organic residues), and (iii) take care to not overseed pots (a rate of 50-60% of first parent culture seems to suffice). Reseeding generally cannot be carried out for more than two propagation cycles because too many roots accumulate in the pot

6a. If sporulation is low or new cultures cannot be started from spores, then carry out a transplantation step (see below) using 1/6 to 1/8 of the pot volume as starter inoculum.

6b. If sporulation is adequate and spores are able to successfully form new mycorrhizae in seedlings, then restart cultures from extracted spores.

Transplanting

1. Starter inoculum either consists of the contents gently removed from a cone-tainer after 4 months growth (with no disturbance) or a section of contents removed from a pot (not shown). Cone-tainers are thin-walled and thus pliable enough to facilitate easy removal of contents without much disturbance. We generally use a surface-sterilized knife to cut the section from a pot to minimize disturbance.

click photo for larger image

2. Fill 15-cm diameter (or larger) pot with sterile growth medium. Create a fairly large hole in the center (we use a large glass rod; even a stirring rod will do) and carefully place either the cone-tainer or pot section contents with attached intact and healthy plants into this hole.

3. Seed all of the surface around the transplant and grow in pot for 4-5 months.

4. To maintain this culture without harvesting, then follow the steps for reseeding discussed above.