امراض النبات Plant Pathology

[الصباح النجار]

In 1972, Johnson and Curl published Methods for Research on the Ecology of Soil-Borne Plant Pathogens. For many years, it was the only book on research techniques focusing on soilborne pathogens. Their perspective was broad, presenting techniques for soilborne pathogens, including fungi, bacteria, and viruses. Many of those techniques are still widely used and will continue to be for years to come. By the late 1970's, the book was no longer in print, and copies are now very difficult to obtain. Dhingra and Sinclair (1985) published Basic Plant Pathology Methods, a book even broader in scope than Johnson and Curl's in covering methodology for both foliar and soilborne pathogens. In 1987, the need for an updated, comprehensive work focused on methods for working with soilborne fungal plant pathogens became clear to members of the American Phytopathological Society Soil Microbiology and Root Disease Committee. Thus, after several years of discussion, the effort to develop a new book was finally initiated. Individuals with expertise in soil science, specific soilborne fungi, or other fields pertinent to the study of soilborne plant pathogens were invited to contribute chapters to this publication.
The editors believe the information presented here to be a compilation of the most recent, comprehensive methodology available to those working with soilborne fungal pathogens. Hopefully, it will complement previously published books and help researchers overcome some of the common problems encountered when working with soilborne phytopathogenic fungi. It would also be desirable for this book to lead to greater standardization of methods and techniques used when working with these soilborne pathogenic fungi.
ORGANIZATION
This book is composed of three sections. Section I, in addition to the introduction and organizational information, includes brief reviews of general techniques useful in the study of soilborne phytopathogenic fungi. With the exception of the chapter by J. C. Correll on the use of new molecular techniques for identification of soilborne fungi, the information in Section I is not intended to be detailed or specific. The authors and editors have assumed that the reader is familiar with the basic concepts and principles of plant pathology.

Section II is composed of 30 chapters which focus on specific genera (or groups of genera) of soilborne fungi. Each chapter includes information on Identification, Host Range and Distribution, Isolation, Isolate Maintenance and Storage, and Inoculum Production and Pathogenicity Determinations. A uniform format was used throughout the book. Most authors were instructed to limit their chapters to approximately 10 double-spaced, typewritten pages. Additional pages were allowed for more complex genera such as Bipolaris, Fusarium, Phytophthora, Pythium, and Rhizoctonia. Although each author was restricted by page limitations, the information provided is sufficient to allow an individual with no prior knowledge of a particular pathogen to read the appropriate chapter and begin work without further literature review. To this end, authors were requested to select techniques which they felt were the easiest and most dependable, and to cite other related techniques. This approach required each author to make difficult decisions regarding what to include and cite, but also resulted in an excellent Literature Cited section for each chapter. The number of literature citations was not restricted, and the editors believe that this constitutes one of the real strengths of this book. At the end of the book, complete recipes for a variety of culture media are given in Appendix A. These recipes are organized into sections following the order of the chapters in Section II.
Section III includes basic information on subjects such as soil physical properties, soil temperature, soil moisture, and soil atmosphere. The material in Section III is unique for a plant pathology methods book. Several of the chapters were written by scientists from other disciplines, and much of the information is not specific to plant pathology. However, anyone who works with soilborne pathogens should recognize the importance of the soil environment in which pathogens survive. Section III will help the researcher appreciate many of die complex environmental parameters which affect these fungi and the diseases they cause. The chapters in Section III complement the information in Section II, and together provide sufficient information to begin research on many of the more economically important soilborne fungal pathogens.

Communicate in the upcoming series

C. M. Rush, J. D. Mihail, and L. L. Singleton
Texas Agricultural Experiment Station Bushland, Texas 79012
Department of Plant Pathology University of Missouri, Columbia, Missouri 65211
Department of Plant Pathology Oklahoma State University, Stillwater, Oklahoma 74078

الموضوع الأصلي: امراض النبات Plant Pathology // الكاتب: الصباح النجار // المصدر: خير بلدنا الزراعي

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[الصباح النجار]

SOIL AND PLANT SAMPLING TECHNIQUES
x,^> Soilborne fungal pathogens and the diseases they cause are inherently difficult to study because of the environment in which they are found. The infected root is not readily visible, and aerial disease symptoms are often similar to those caused by other factors such as flooding, drought, nutrient deficiency, soil compaction, insects, and herbicide misapplication. Therefore, before a given symptom can be positively attributed to a soilborne fungal pathogen, soil and/or root samples must be obtained. The following sections include general information that should be considered when sampling. More detailed information can be found in the chapters by W. L. Bland and K. B. Johnson in Section III.
Plant sampling- Two basic questions to consider when sampling are: "When did the plant become infected?" and "What part of the plant should be collected?" To answer these questions, it is important to have some understanding of both the pathogen and the disease of interest. Pathogens causing seedling diseases frequently infect their host(s) soon after seed germination. These same fungi may be essentially nonpathogenic to older plants. Likewise, some pathogens only infect mature plants and not seedlings. This phenomenon may represent a true difference in host-tissue susceptibility over time, or merely illustrate the importance of specific environmental conditions required for host infection and disease development. Regardless of plant age, if the purpose of plant sampling is to isolate a suspected pathogen, one should sample as soon as disease symptoms appear or even before. It is usually difficult to isolate pathogens from plant tissue in advanced stages of decay. If the purpose of sampling is to determine when infection occurs, it should be initiated long before any disease symptoms appear. Many soilborne fungi infect plants soon after seedling emergence, but disease symptoms are not expressed until the plant experiences some type of environmental stress such as heat or drought.
The second question (i.e., what part of the plant should be collected) also depends on the specific purpose of the sampling. Again, it is helpful to have some preliminary information on the pathogen and disease. Soilborne fungal pathogens are often localized or restricted to a particular part of the root such as the vascular system, cortex, or root tips. Attempts to detect or isolate a specific pathogen can be frustrating if the wrong plant tissue is sampled. For instance, Polymyxa betae Keskin, the vector of beet necrotic yellow vein virus, is restricted to cortical tissue and will not be found in older lateral roots or in the sugar beet tap root. Observation of these tissues could lead to the erroneous conclusion that Polymyxa was not present in a root sample. Such a wrong conclusion or diagnosis could have serious consequences.
When sampling to isolate a root-infecting fungal pathogen, isolation from root samples is not always the best choice. Even though the fungus may be isolated from roots, it may be easier to obtain pure cultures from other portions of the plant. An example of this is Bipolaris sorokiniana (Sacc.) Shoemaker, the cause of common root rot of wheat, which can be isolated very easily from the subcrown internode. Aphanomyces cochlioides Drechs. is best isolated from the hypocotyl of diseased sugar beet seedlings. Several vascular wilt pathogens

can be isolated from aboveground plant parts such as stems and leaf petioles. In this regard, it is important to be aware that different fungal species or anastomosis groups (AGs) of Rhizoctonia solani Kuhn, may predominate on a particular portion of the plant. On sugar beet, AG-4 is the predominant seedling pathogen, but older beets are mainly infected by AG2-2. Similarly, in wheat, AG-8, the cause of bare patch, mainly infects young roots and root tips, whereas AG-4 infects the crown and lower stem and leaf sheaths.
One should be open-minded when first sampling plants for purposes of pathogen isolation and identification. Producers are often acutely aware of disease problems, but frequently group them all together under the generic designation of "rot." There is always a possibility that unidentified pathogens are present and responsible for disease symptoms thought to be caused by another pathogen. If an individual begins sampling with a preconceived idea of the cause of the problem, the true causal agent might be overlooked. When possible, entire plants should be sampled with as much of the root system intact as is reasonably possible. In addition, apparently healthy plants also should be included when sampling, for comparison purposes.
Soil sampling- Soil sampling is usually done to determine the presence, inoculum density, or distribution of a particular pathogen. As with root sampling, timing is an important factor to consider. Pathogen populations are dynamic, both quantitatively and qualitatively. For instance, many pathogens, such as Phymatotrichwn omnivorum (Shear) Dugger, Sclerotium rolfsii Sacc., and R. solani, overwinter as sclerotia or some other dormant form in relatively low numbers. However, during the growing season when a susceptible crop is in the field, these fungi can achieve high populations as mycelium growing through the soil and colonizing host tissue or crop residues. Because fungi occur in various forms in the soil, inoculum or fungal density is often expressed as colony forming units per weight or volume of soil (i.e., CFU/g or CFU/10 mm3), as opposed to a more specific designation of fungal structure such as oospores, conidia, or chlamydospores. The fact that various forms do predominate at different times is important, however, because they can differ in pathogenicity (i.e. inoculum potential) and in their ability to survive storage.
Once sampling time has been determined, the actual process, while possibly labor intensive, is usually simple and straightforward. Numerous tools and devices have been developed for soil sampling, but the best one to use depends on the depth at which the sample must be taken, the volume of soil required per sample, and the total number of samples needed. Perhaps the most difficult part of soil sampling is determining how many samples must be taken, and preventing cross contamination between samples. This issue is especially important when sampling soil from different depths or across a large field with potentially different soil types. The following section includes information on statistical considerations when sampling.
Sampling strategy- If an investigator wishes to determine the amount of inoculum in a field, it is necessary to sample the soil. Although the mechanics are straightforward, one is immediately faced with determining the appropriate number of samples and their arrangement in the field, since fungal inoculum is not uniformly distributed throughout a field (Campbell and Noe, 1985). Several recent studies have focused on the problems associated with sampling soil in order

4

to estimate the populations of soilbome fungi (Lin et al, 1979; Mihail, 1987). These studies have compared various methods of arranging sampling sites within a field. The simplest is to walk along a diagonal path from one corner of the field to the opposite corner and take 10-20 samples equally spaced along the path. However, this approach does not distribute the sampling sites well over the field (Lin et al, 1979; Mihail, 1987). A more effective approach is to traverse a "diamond" or "W" shaped path through the field, collecting 20-30 samples equally spaced along the path (Lin et al, 1979; Mihail, 1987). Once samples are collected, they may be bulked prior to assay, however, this does not permit the investigator to estimate the variability in pathogen population occurring within the field. If the samples are assayed individually, a mean and variance may be estimated for the pathogen population. However, these two measures do not provide information concerning the spatial pattern of the inoculum. If information of this type is desired, the reader should consult the review article of Campbell and Noe (1989) or studies of spatial pattern with specific soilborne fungi. The consideration of sampling strategies as they relate to crop loss assessment is treated in the
chapter by K. B. Johnson

Communicate in the upcoming series

.

[الصباح النجار]

ISOLATION AND IDENTIFICATION OF PATHOGENS
Once plant and soil samples have been collected, isolation and identification of the pathogen is the next task facing the investigator. To isolate a soilborne fungus from host tissue, the investigator must first decide upon the appropriateness of surface-disinfestation of the tissue. For large pieces of woody tissue (i.e., large tap roots), surface-disinfestation is often necessary to prevent the growth of surface-resident saprophytic 2*^1 fungi which might prevent the growth of the pathogen. However, for fine feeder roots, surface-disinfestation may kill pathogens such as Pythium spp. inside the roots g The choice of a surface-disinfestation treatment and the duration of the treatment will vary with the different groups of fungi. The next step in the isolation of the fungus from host tissue is the selection of an appropriate culture medium. Appendix A lists a number of general and highly specific media for this purpose. The isolation of soilbome pathogens from soil can employ soil-dilution plate techniques, selective (or semi-selective) . V-*, media, or baiting. In general, the soil-dilution plate technique (. (Tuite, 1979) involves drying the soil sample, followed by ' crushing it through a 2-mm sieve. A 10-g subsample is added .to 200 ml of 0.2% water agar (WA) (or 1% sodium carboxymethyl cellulose) in a screw-capped bottle. The ! contents are mixed thoroughly for 20jnin, then a 1-ml aliquot is withdrawn and added to 9 ml of 0.2% WA (or other diluent) and shaken for 4 min. A 1-ml aliquot is removed and added to 49; ml of 0.2% WA and shaken for 2 min. Using a wide-mouth pipette, transfer 1 ml of the final dilution to each of five sterile petri dishes and add 17 ml of the desired culture medium which has been cooled to 45C. Disperse soil particles by circular agitation of the petri dishes. The petri dishes are incubated under conditions appropriate for the fungus of interest. This description is offered only as a general illustration of the technique, and the actual amount of dilution of the soil sample will depend upon the number and type of fungal propagules present. If many are present (i.e., 10s CFU/g) then a higher dilution will be required than where the fungal population is less than 10 CFU/g.

A commonly used variant of the soil-dilution plate technique is the Warcup plate method (Tuite, 1969; Warcup, 1950) wherein a small soil sample (0.005 - 0.15 g) is transferred to a sterile petri dish and crushed in a drop of water. To the petri dish, add 8-10 ml of the desired growth medium. Gently swirl the plate to distribute the soil particles in the medium and incubate as appropriate for the particular fungus. Tuite (1969) recommends Czapek's agar (Appendix A) amended with 0.5% yeast extract and acidified to pH 4.0 with phosphoric acid.
Many selective media have been devised for the recovery of soilborne fungi from soil samples. In principle, they all involve the addition of various antimicrobial chemicals to suppress the growth of other organisms which might interfere with the target organism. As a cautionary note in using selective media, the investigator should be aware that each selective medium was devised for use with one (or a limited number) of soil types. Thus, a medium which works perfectly well in Texas may perform poorly when used in Missouri.
As an alternative to selective media, several investigators have used plant tissue as "bait" to isolate plant-pathogenic fungi (i.e., Pythium and Phytophthora spp.) from soil. The bait tissue is selected because it will selectively permit the growth of the desired fungus.
Once the putative pathogen has been recovered in pure culture, the investigator is faced with the task of identifying it. The prerequisite for fungal identification is the production of all taxonomically useful structures for microscopic (or macroscopic) examination. For the Deuteromycotina, it is possible to induce many of these fungi to produce reproductive structures on microscope slides using the Riddell slide culture technique (Riddell, 1950). A 1-cnf square of potato dextrose agar (PDA, Appendix A), or other suitable culture medium, is aseptically placed in the center of a sterile glass microscope slide. A 2-mm2 inoculum-block of the fungus is aseptically placed at the center of each of the four edges of the agar square. A sterile cover slip is then applied to the agar square and the entire slide culture is incubated in a moist chamber under conditions appropriate for the particular fungus. When fungal growth has extended over several mm from the original inoculation sites, the cover slip is lifted off vertically, a drop of lactophenol (Appendix A) or other mounting medium (or stain) is added to the culture, then the cover slip is inverted and gently placed on a clean microscope slide. This first culture is now ready for microscopic examination. The 1-mm2 agar block is gently removed from the original microscope slide culture. Suitable mounting media or stains are applied, followed by gentle addition of a cover slip to complete the preparation of the second culture.
Ultimately, identification of a particular fungus will require consultation with an appropriate monograph (or with an appropriate expert). However, there are several general mycological texts which may aid in identification. These include Hawksworth 1974, Hawksworth et al, 1983, and Domsch et al, 1980.

[GOGO KEWAIS]

انجليزى ده ميرسيى
هههههههههه
صدقنى مجهود
راااااااااااائع تسلم ايديك

[م/ إيهاب عبد المؤمن]

موضوع متميز للغاية ومرتب وبحث ذات أهمية كبيرة للجميع وليس المتخصص فقط .

تحياتي الغالية لك أخي الصباح .

[الصباح النجار]

Gogo &Abu hazem
many thanks for you about your
comments.iam very pleasure for that.
thanks again& Best Regards