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MECHANISM 0F INCREASED SUSCEPTlBiLiTY 0F
BLEACHED PEA SEEDS T0 SEED AND SEEDUNG ROT

Thesis for the Degree of M. S.
WCHIGAN STATE UNIVERSlTY
ROSEMARY LORIA
1977

    
     

  

L I" 32 A R Y
Mike}; :5 :1 53358
Umversity

   

Q/oztm/

ABSTRACT

MECHANISM OF INCREASED SUSCEPTIBILITY OF

BLEACHED PEA SEEDS TO SEED AND SEEDLING ROT

BY

Rosemary Loria

Maturation of pea (Pisum sativum L. 'Miragreen') seeds during

 

moist, hot, sunny weather causes many green pea seeds to turn yellow.
This process, known as bleaching, has been reported to increase seed and
seedling rot of peas in growth chamber studies. Bleached and nonbleached
seeds were placed in beds of glass beads in the laboratory, inoculated

with l x 108 conidia of Fusarium solani f. sp. pisi per seed. Some

 

seeds were leached with distilled water. Disease severity of leached
seeds was reduced below that of nonleached controls, apparently due to
the removal of nutrients from the host-pathogen interface. Green seeds
were placed in beds of glass beads, inoculated as before, and exudates
of bleached or nonbleached seeds were added. Seeds incubated in
exudates from bleached seeds had a higher disease rating than those
incubated in exudates from nonbleached seeds. When bleached and non-
bleached seeds were allowed to inbibe water, and conidial suspensions
(10, 100, or 1,000 conidia/seed) were injected beneath the seed coat,
disease severity was similar.

Exudates from bleached and nonbleached seeds contained similar

amounts of ninhydrin-positive substances. Fourteen amino acids were

Rosemary Loria

present in exudates from both seed types; no qualitative or quantitative
differences in the amino acid composition were observed. Bleached seed
exudates contained approximately three times more soluble carbohydrate
than did nonbleached seed exudate. Sucrose, glucose, and fructose were
identified from both types of seed exudate, but all three sugars were
present in larger quantities in bleached seed exudate. Bleached seed
exudate was especially rich in sucrose. When the seed exudates were
fractionated into anionic, cationic, and neutral components on ion
exchange resins, only the carbohydrate-containing (neutral) fraction
stimulated chlamydospores of E, gglani_f. sp. pi§i_to germinate in
natural soil. The neutral fraction of bleached seed exudate caused 40%
of the chlamydospores to germinate while the same fraction of nonbleached
seed exudate promoted 10% germination. When a 0.1 M solution of sucrose
was applied to inoculated nonbleached seeds, disease severity was in-
creased over distilled water controls.

Pea seeds were planted in the field in ten footrows, in soil
artificially infested with E, §91§2i.f- sp. pi§i_chlamydospores. Plots
planted with nonbleached, partially-bleached, and bleached seeds had 69,
58, and 31% emergence, total fresh weights (grams of stems, leaves and
pods) of 2398, 1965, and 1327, and shelled pea weights (grams) of 477,
445, and 237 per plot, respectively. Since the three types of seeds were
equally viable when germinated in vitro, these data indicate that
bleaching appears to increase the susceptibility of pea seeds to seed and
seedling rot in the field. Differences in carbohydrate (especially
sucrose) exudation from bleached and nonbleached seeds is probably the

basis for differences in seed and seedling susceptibility to E, solani

f. sp. pisi.

MECHANISM OF INCREASED SUSCEPTIBILITY
OF BLEACHED PEA SEEDS TO SEED AND

SEEDLING ROT

BY

Rosemary Loria

.A THESIS

Submitted to
‘Michigan State University
in partial fulfillment of the requirements
for the degree of

iMASTER OF SCIENCE

Department of Botany and Plant Pathology

1977

To Lenny,

my best friend

ii

ACKNOWLEDGEMENTS

To Dr. Melvyn L. Lacy, I express appreciation for his guidance
during this project, and for his assistance in the preparation of this
manuscript.

To the members of my guidance committee: Dr. John L. Lockwood,
and Dr. Donald C. Ramsdell, I extend my thanks for their suggestions and
critical evaluation of the manuscript.

I especially want to thank Lenny for his faith, inspiration,

and patience.

iii

TABLE OF CONTENTS

LIST OF TABLES

LIST OF FIGURES .

INTRODUCTION .

LITERATURE REVIEW

METHODS

RESULTS

AND MATERIALS .

Maintenance of the pathogen and
preparation of inoculum

Source and preparation of seeds .

Source, preparation, and infestation
of soil .

The leaching apparatus .
Inoculation of seeds by injection
Evaluation of disease

Collection of exudates .
Fractionation of exudates .
Chemical analysis of exudates

Chlamydospore germination .

Emergence, fresh weight, and seed
viability . . .

Influence of exudates on infection .
Chemical analysis of seed exudates .
Chlamydospore germination .
Influence of sucrose on disease

incidence

iv

vi

. vii

10

12
12
14
14
14
15
16
17
18

18
20
23

26

32

DISCUSSION

LITERATURE CITED

36

41

LIST OF TABLES

Table

1.

10.

11.

Comparison of two surface-sterilizing agents on carbo—
hydrate exudation from bleached Miragreen pea seeds in
moist glass beads . . . . . . . . . .

Effects of seed bleaching and seed treatment on
emergence, fresh weight, and yield of Miragreen peas

Effects of seed bleaching and seed treatment on the
fresh weights and yields of individual pea plants

grown from nonbleached, partially-. bleached, or bleached
Miragreen pea seeds . . . . . . .

Effect of leaching with distilled water on infection of
bleached or nonbleached seeds by E, solani f. sp. pisi .

Effect of exudates from bleached or nonbleached pea
seeds on infection by F. solani f. sp. pisi of non—
bleached pea seeds in sterile, moist glass beads .

Effect of injection of bleached or nonbleached Miragreen
pea seeds with conidia of E, solani f. sp. pisi

Exudation of carbohydrates and ninhydrin-positive sub-
stances from pea seeds incubated for 5 days in a moist,
sterile, sand environment at 22°C .

Carbohydrates exuded from bleached and nonbleached pea
seeds . . . . . . . .

Amino acids exuded from bleached and nonbleached pea
seeds . . . . . . . . . . . .

Stimulation of F. solani f. sp. pisi chlamydospore
germination in natural soil by bleached or nonbleached
pea seed exudates, or components of these exudates

Effect of exogenously applied sucrose on infection of
nonbleached pea seeds by E, solani f. sp. pisi

vi

Page

11

19

21

22

24

25

27

28

31

33

3S

LIST OF FIGURES

Figure Page

1.

Apparatus used for leaching pea seeds. Ten seeds were

placed in the bed of glass beads, and the peristaltic

pump supplied 75 ml of water .during a period of fifteen

minutes every hour . . . . . l3

Representation of a thin layer chromatogram: l, bleached

seed exudate (20 ul); 2, unbleached seed exudate (40 ul);

3-10, standards sugars (10 ug each). The colors produced

by the detector are depicted in the following manner:

0 = red-brown; 6 = green; 0 = brown; 6 = gray-brown . . . . 29

Gas chromatogram of'DMS derivatives of carbohydrates

from bleached pea seed exudate. Peaks are: l, fructose;

2, unknown; 3 and 4, glucose; 5, inositol (internal

standard); and 6, sucrose. Chromatographs of’DWS

derivatives of carbohydrates from nonbleached pea seed

exudate did not differ qualitatively from this one . . . . 30

vii

INTRODUCTION

Pea seed viability and seedling vigor appear to depend on
environmental conditions during seed maturation, and on a timely
harvest (31). Maturation of pea seeds during moist, hot sunny weather
causes many green seeds to turn yellow, a process known as bleaching
(29). Bleached seeds are of questionable value as seed, since there is
evidence that they may be more susceptible to seed and seedling-infect-
ing fungi than nonbleached seeds of the same variety (55).

Germinating pea seeds exude nutrients such as sugars (17, 29,
54) and amino acids (51) which diffuse into the spermosphere soil (56).
These nutrients stimulate spore germination and vegetative growth of
the spermosphere microflora, including seed-infecting fungi. Exudates
from germinating bleached seeds contained more carbohydrates than
exudates from germinating nonbleached seeds (29, 54). Preemergence
damping-off and carbohydrate exudation were higher among wrinkled-
seeded pea cultivars than among smooth-seeded pea cultivars (l7).
Carbohydrate exudation was also a determining factor in the suscepti-
bility of some soybean varieties to Eythium infection (25).

Amino acids are also components of pea seed exudates (51).
Those from pea apparently have not been evaluated as stimulants of
germination of pathogens of pea seeds, but those from other plants
have. For example amino acids from bean and pine seeds have the

ability to stimulate germination of chlamydospores of Fusarium solani

 

2

f. sp. phaseoli (52), and zoospores of Pythium afertile (3), respec-

 

tively. Amino acids or other nitrogen-containing compounds in tomato
root exudate may be responsible for stimulating germination of conidia

and microsclerotia of Verticillium albo-atrum in soil (46). Conidia of

 

E, §21§El.f° sp. phaseoli were more virulent to bean stems when
supplied with organic sources of nitrogen than when supplied with only
glucose (61). Both organic and inorganic sources of nitrogen increased
the incidence of the root disease of bean caused by E, gglagi f. sp.
phaseoli under field conditions (69).

The evidence suggests that the increased nutrients in exudates
from bleached, as compared with nonbleached pea seeds, may cause in-
creased seedling susceptibility to E, gglagi_f. sp. pigi, The objec-
tives of this study were to determine if nonbleached pea seeds are more
resistant to E, E91§21.f' sp. pi§i_than bleached pea seeds in the
field, to investigate the role of seed exudates in the differences in
susceptibility expressed by nonbleached and bleached seeds, and to
determine the effect of some components of pea seed exudate on chlamy—

dospore germination and pathogenesis of E, solani f. sp. pisi.

LITERATURE REVIEW

Exudation of nutrients from germinating seeds and roots is
known for a number of plant species, and is probably common to all
higher plants. Although there have been extensive investigations of
the composition of exudates from plant roots (5, 24, 62, 63, 64, 65,
66), few data are available on the composition of exudates from germin-
ating seeds. There is ample evidence that carbohydrates, as a class,
are present in the seed exudates of peas (26, 32, 33, 34, 51, 54, 57),
beans (25, 47, 51), and cotton (51), and that amino acids or related
compounds are found in bean (42, 47, 51), cotton (51), and pea (51)
seed exudate. In addition, specific compounds have been identified
from seed exudates: several sugars and amino acids from cotton (19),
pine (3), and bean (28, 52), and aliphatic and aromatic acids from
cotton, pea, and barley (27).

The relation of seed and root exudates to relatively high
microbial activity in the soil around these structures, termed the
spermosphere (67) or rhizosphere (21), is well documented. These
exudates influence pathogenic fungi directly by inducing germination,
enhancing nutritional status before penetration, and inhibiting growth;
or indirectly by stimulating competition or antagonism from other
microorganisms (49). Therefore, the kinds and amounts of substances
exuded from seeds or roots have a strong influence on host-pathogen

interactions in the spermosphere or rhizosphere.

Effect of Exudates
on Spore Germination

 

 

Propagules of seed and root-infecting fungi remain.dormant in
soil until stimulated to germinate by a nutrient source (10, ll, 18,
56). In most cases this stimulatory effect is nonspecific, and there
are many reports of dormant fungal propagules germinating in the rhizo-
sphere of nonsusceptible plants (46, 48, 58). The ability of various
components of seed or root exudates to stimulate germination of dormant
fungal propagules has been investigated. Conidia and microsclerotia of

Verticillium albo-atrum in natural soil were stimulated to germinate by

 

the basic fraction of tomato-root exudate, which contain amino acids,
but not by the neutral-acidic fraction, which contains sugars and
organic acids (46). Since sugars have been shown to stimulate germina-
tion of microsclerotia in soil (16), the lack of germination in
response to the neutral-acidic fraction may have been due to a level of
carbohydrate in the exudate lower than that necessary to stimulate
germination, or to an inhibition of germination by organic acids in the
exudate. Organic acids have been reported to inhibit zoospore germina-

tion of Eythium afertile (3).

 

All sugars and most amino acids identified from seed exudates

of Pinus resinosa stimulated zoospore germination of Pythium afertile

 

 

when supplied singly; glucose and asparagine were particularly
effective in accelerating germ tube development (3). Exudates were
collected from germinating bean seeds, and amino acids and sugars were
identified and assayed individually for their ability to stimulate
germination of chlamydospores of E, gglggi f. sp. phaseoli in soil.

While all sugars and most amino acids stimulated germination to some

degree, glucose and asparigine stimulated chlamydospore germination to a

greater extent than any of the other components tested (52).

Effect of Exudates on
Competition and Antagonism

 

 

Seed and root exudates stimulate microorganisms which are
antagonistic to pathogenic fungi in the spermosphere or rhizosphere.
Slykhuis (59) found that the number of bacteria in soil apart from
grass seeds was not correlated with the amount of suppression of
Fusarium blight, while the numbers in 5011 around germinating seeds was.
The primary mechanism.by which 5011 bacteria inhibited E, ogysporum‘was
by immobilization of nitrogen when the carbon supply was high (30).
This inhibition was removed when the ratio of carbon to nitrogen was
less than five. The ability of bacterial isolates to compete with E,
ogysporum.was not related to their growth rates, but was correlated
with their ability to develop in the absence of growth factors.

Soil moisture influences the survival of germinated spores by
affecting bacterial activity. In soil amended with carbon and
nitrogen, chlamydospores of E, :9gggm_f. sp. cerealis 'Culmorum' germ-
inated and grew well at soil water potentials below 10 bars (13). At
higher water potentials, germ tubes lysed due to high bacterial
activity. When antibiotics were added to the soil with the nutrients
the germ tubes did not lyse, even at the highest water potential tested
(-l.0 bars). In soil near pea seeds, high soil water potentials in-
creased germination of chlamydospores of E, §91§§i_f. sp. pi§i_due to
increased seed exudation. Soil water potential also influenced germ-
ling survival by modifying bacterial activity (12). In soil containing

more than 8.7% moisture, germination at 20 hours after planting was

high; but by 48 hours up to half of the germ tubes were lysed. In
drier soils, germination was lower but no lysis was detected. The
number of germ tubes that successfully penetrated the foot region of
the plant was greater at 8% soil moisture than at all other moisture
levels tested.

Effect of Exudates on
Disease Incidence

 

 

There is ample evidence for a relationship between seed and
seedling exudation and susceptibility of seedlings to damping-off
diseases. Resistance of soybean varieties to preemergence mortality
caused by Eythium was negatively correlated with the amount of carbohy-
drate exuded from the germinating seed (25). When the seeds of a
resistant variety were coated with powdered sucrose and planted in
infested soil, preemergence mortality was increased. The quantity of
electrolytes leaching from seeds of 11 cultivars of pea or 16 cultivars
of french bean that were soaked in distilled water was directly related
to the incidence of damping-off in the field (33). In the same study,
the amount of soluble carbohydrate exuded from.pea seeds was also
correlated with preemergence mortality in the field. There was a
direct relationship between preemergence damping-off of three bean
varieties and the quantity of fluorescent, ninhydrin-positive, and
silver nitrate-positive substances in the seed exudates (47). Flentje
and Sakena (17) found that susceptibility of wrinkled-seeded peas to
Eyghium was due to high quantities of carbohydrates in the seed exudate.
Smooth-seeded peas which exuded small quantities of carbohydrates were
resistant to the damping-off disease caused by this fungus. The in-

cidence of foot-rot disease of rice caused by E, moniliforme was

 

reduced when germinated, rather than ungerminated, rice seeds were sown
in infested soil (44). Most of the nutrients had been exuded from the
seeds before they were planted, and therefore were not available to
increase inoculum potential. Kerr (26) found that the effect of soil

moisture on infection of peas by Pythium ultimum was due to its

 

influence on seed exudation, More sugar was exuded from germinating
peas at higher soil moistures, and the amount of sugar in the seed
exudate was directly related to disease incidence.

Temperature has been shown to influence exudation from seeds
and roots. An increase in amino acid exudation from strawberry roots at

low temperatures increased the severity of Rhizoctonia root decay (22).

 

Seven and three times as much total amino acids and sugars were exuded
at 18 and 24°C, respectively, than at 30°C by germinating cotton seeds
(19). Evidence suggested that this increase in seed exudation at low
temperatures was associated with the preemergence mortality of cotton
seedlings caused by E, solani under these conditions. Vancura (63)
observed that 'cold shock' stimulated higher exudation from the roots
of maize and cucumber. An increase in the number of fungi in the
spermosphere of maize was also observed after exposure to low tempera-

tures (53).

Bleaching of Seeds

 

Extremes of temperature, moisture, and light following seed
maturation result in a loss of chlorophyll from the cotyledons of peas
(29), lhma beans (43), and other species (40), a process known as
bleaching. There were no differences in the constituents of bleached
and nonbleached pea seeds when.mineral composition (6), amino acids,

sugars, and carboxylic acids (29) were examined. However, exudates

from germinating bleached seeds have been shown to contain more carbohy-
drates than exudates from germinating nonbleached seeds (29, 54). Other
components of the exudates from bleached and nonbleached seeds appar-

ently have not been compared.

MATERIALS AND METHODS

Maintenance of the Pathogen
and Preparation of Inoculum

 

 

A culture of Fusarium.solani (Mart.) Sacc. f. sp. pisi (Jones)

 

Snyder 8 Hansen isolated from.Pisum sativum L. was obtained from J. L.

 

Lockwood,.Michigan State university, and maintained on potato-dextrose
agar petri plates (PDA) at 24°C under continuous fluorescent light.
Conidia were harvested by flooding colonies with 10 ml of sterile dis-
tilled water, then washing the conidia by centrifugation in three
changes of sterile, distilled water. The pelleted conidia were re-
suspended in sterile distilled water and the concentration was adjusted
as necessary using a hemacytometer. Chlamydospores were produced in
shaken culture as follows: Conidia, prepared as described above, were
incubated in potato-dextrose broth (PDB) for 24 hours, centrifuged,
washed, and placed in agitated, sterile aqueous soil extract for 10-14
days (prepared by mixing 1 liter Conover loam soil with one liter of
water, allowing to stand for 48 hours, and filtering the supernatant
through a 2.2-um Gelman membrane filter). Chlamydospores formed by
macroconidia were then washed by centrifugation and agitated at a low
speed in a Sorvall Omni4Mixer for 1 hour to break up chlamydospore
aggregates. The concentration of chlamydospores was adjusted as

necessary using a hemacytometer.

10

Source and Preparation
otTSeeds

 

A wrinkled-seeded pea (Pisum sativum L. cv. Miragreen)

 

obtained from Ferry—Morse Seed Company (1974 seed lot) or grown at the
Michigan State university Botany Farm (1975 seed lot) was used. Indi-
vidual seeds were selected on the basis of uniformity in size and
freedom from spots or cracks on the seed coat, then sorted according to
the degree of bleaching into lots of bleached and nonbleached. Sodium
hypochlorite (NaOCl) is widely used for surface sterilizing seeds in
exudate collection studies (3, 19, 27, 54). However, there is evidence
that NaOCl may effect seed metabolism, and that it cannot be removed
with distilled water (1, 2). Exudation of soluble carbohydrate from
bleached pea seeds (1974) that had been surface sterilized with 1% NaOCl
for 30 minutes was compared with that from seeds sterilized with 30%
hydrogen peroxide (H202) for 5 minutes. These treatments provide equiva—
lent degrees of surface sterilization. The seeds were treated as
described, rinsed with three changes of sterile distilled water, and
incubated in leaching dishes (a modified deep petri dish, with an outlet
in the lower half of the dish, containing 300 g of moist 1 mm-diameter
glass beads) for 24 hours at 22°C. The exudate was collected by flush-
ing the beads with two 50 ml aliquots of sterile distilled water. The
exudate was passed through a 2.2 pm Millipore filter, taken to dryness in
a flash evaporator at 60°C, and redissolved in 10 ml of distilled water.
Total soluble carbohydrate was determined with a modified anthrone
analysis (39) using a standard curve derived from glucose. Seeds steril-
ized with NaOCl exuded more soluble carbohydrate than those sterilized
with H202 (Table 1). It was concluded that H202 was a.more desirable

surface sterilant than NaOCl for seed exudation studies. For experiments

11

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12
requiring aseptic conditions, seeds were treated for 5 minutes in 30%

H202, followed by 3 rinses in sterile distilled water.

Source, Preparation, and
Infestation of Soil

 

 

Conover loam soil from the Michigan State University Botany
Farm, from an area free from recent pesticide application, was used for
field as well as laboratory experiments. Prior to use in laboratory
studies, the soil was air—dried and passed through a 30-mesh sieve, then
stored in covered metal containers lined with plastic bags. Soil in-
fested with chlamydospores of E, gglggi f. sp. pi§i_was obtained for
laboratory experiments by placing air—dried, sieved soil in a small
rotary mixer with baffles, and applying an aqueous spore suspension with
an atomizer until the desired spore concentration and soil moisture were
attained. Field soil was infested by spraying a suspension of chlamydo-

spores into the seed furrow after planting but prior to covering seeds.

The Leaching Apparatus

 

.A leaching system was employed which consisted of a modified
deep petri dish, with an inlet in the lid and an outlet in the lower half
of the dish, containing 300 g of l mm-diameter glass beads (Figure l).
Sterile distilled water was pumped from a reservoir to the leaching dish
by a peristaltic pump. The water passed through the dish and into a
drainage flask. Ten yellow or green seeds were placed in each leaching
system. The seeds were then individually inoculated with 1 ml of a
conidial suspension (1 x 108/ml) of E, §91§§i_f. sp. pi§1_and covered
with glass beads. The peristaltic pump supplied 75 ml of water over a
period of fifteen minutes during each hour. Noninoculated seeds served

as controls.

13

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14

Inoculation of Seeds by Injection

 

Surface-disinfested bleached and nonbleached seeds were allowed
to imbibe water for 24 hours on moist filter paper in petri dishes.
Seeds were then injected in one of the cotyledons with 1 ul of a
conidial suspension containing 10, 100, or 1,000 conidia respectively,
using a 10 ul Hamilton syringe which had been sterilized in 95% ethyl
alcohol and rinsed in sterile distilled water. Noninjected seeds and

seeds injected with sterile distilled water served as controls.

Evaluation of Disease

 

Seeds were incubated at 22°C for five days unless otherwise
noted, then evaluated for disease severity. A rating system of 0 to 5
was used: 0 indicated no lesions; 1 = 1% to 10% of the seed was
necrotic; 2 = 11% to 25% of the seed was necrotic; 3 = 26% to 50% of the

seed was necrotic; 4 = 51% to 75% of the seed.was necrotic; and S = > 75%

of the seed was necrotic.

Collection of Exudates

 

Twenty-five mm-diameter test tubes were filled with 25 g of
acid—washed silica sand. Four ml of glass-distilled water was added to
each tube, and the tubes were capped and autoclaved. Miragreen pea seeds
(1975) were prepared as described. One yellow or green seed was put into
each tube and covered with 10 g of sterile sand. Three ml of sterile
distilled water was added to each tube, and the tubes were sealed with
Parafilm (American Can Company) and incubated at 22°C for 5 days. The
seeds were then removed from the tubes and placed on PDA plates for 5
days. TUbes which contained contaminated seeds were discarded. The sand
from the remaining tubes was washed with glass-distilled water, the

leachate was filtered through a Gelman membrane filter (2.2 um pore

15

size), evaporated to dryness in a flash evaporator at 60°C, and re-
dissolved in 10 ml of glass-distilled water. This exudate solution was

stored at —20°C until used.

Fractionation of Exudates

 

Concentrated solutions of pea seed exudate were fractionated
into cationic, anionic, and neutral components. Thirty ml of cation
exchange resin (Bio Rad AG 50-X8, H+ form) was prepared by passing SN
NaOH through the resin in a 1.5 cm—diameter column until the pH was 14,
rinsing with glass-distilled water until the pH was 5, passing 5N HCL
through until the pH was 1, then rinsing again until the pH was 5.
Thirty ml of anion exchange resin (Bio Rad AG l-X8, formate form) was
prepared similarly, in a column of 1.5 cm-diameter, by rinsing sequentie
ally with 2N NaOH until the pH was 14, glass-distilled water until the
pH was 5, IN acetic acid until the pH was 1, then glass-distilled water
until the pH was 5. Five ml of a concentrated pea seed exudate solution
was applied to the cation exchange column and washed through with 300 ml
of .01 N HCL. The wash from the cation resin was taken to dryness twice,
redissolved in glass—distilled water, then applied to the anion exchange
resin. The anion resin was rinsed with 300 ml of glass-distilled water,
and this solution was designated the neutral fraction. The cation ex-
change resin was eluted with 300 ml of 4 N HCL (cationic fraction), and
the anion exchange resin was eluted with l N acetic acid (anionic
fraction). All three fractions were taken to dryness twice and re-
dissolved in 5 ml of glass-distilled water for chlamydospore germination

studies.

16

Chemical Analysis of Exudates

 

Total water-soluble carbohydrate was determined by a modified
anthrone analysis (39) in.which 1 ml of exudate Was mixed with 9 ml of
anthrone reagent, placed in a boiling water bath for 10 minutes, and
immediately cooled in an ice bath. The solution was then allowed to
warm to room temperature, and optical density at 600 nm was measured
with a Bausch and Lomb Spectronic 20 spectrophotometer. Carbohydrate
concentrations were determined using a standard curve derived from
glucose. Total amino acids and related compounds were determined by the
ninhydrin.method of Moore and Stein (38), using glycine as a standard.

Carbohydrates were separated on thin layer chromatography plates
coated with silica gel (layer thickness 0.25 mm) obtained from.E. Merck
Laboratories Inc., Rahway, N.J. The solvent system used was n—butanol:
acetone: water (4:5:1, v/v/v) and the carbohydrates were detected by
spraying the chromatogram with.ADOP indicator (Aniline, 4 m1; diphenyl-
amine, 4 g; orthophosphoric acid 20 ml in.200 ml acetone mixed with 100
ml acetic acid), then heating for 10 minutes at 100°C (23).

Carbohydrates were also separated and quantified by gas-liquid
chromatography of trimethylsilyl (TMS) derivatives according to the
method of Sweeley et al (60). TMS derivatives of the carbohydrates were
formed in pyridine containing hexamethyldisilazane and trimethylchlorosi-
lane at 22°C in Kimax vials (100 x 13 mm) covered with a teflon-lined
cap. The Hewlett Packard (Model 402) gas chromatograph, with hydrogen
flame ionization detector, employed a U-shaped glass column (2 mm
diameter) packed with 80-100 mesh Gas Chrom Q (Applied Science Labora-
tories Inc.). Separation of the carbohydrates was done using linear
temperature-programmed analysis from l40-240°C at 2°C min'l. The flow

rate of the nitrogen carrier gas was 25 ml min-l. Inositol was used as

17
an internal standard and the detector response factor was calculated
using standards of glucose, fructose, sucrose, and inositol that were
silyated by the same procedure used for the exudates.

Individual amino acids were identified and quantified. Exudate
samples containing 2,000 - 3,000 nm of glycine equivalents per ml were
taken to dryness at 60°C in a flash evaporator, and redissolved in 2.5
ml of 70% ethanol. The samples were then incubated for 12 hours at 10°C
and the precipitate was removed by centrifugation. The supernatant was
taken to dryness at 60°C in a flash evaporator and redissolved in.1 ml of
.01 N HCL. Samples (250 pl) were then run on an amino acid analyzer
(modified Technicon system) which used Chromo Beads C2 (Technicon Corp-

oration, Tarrytown, N.Y.)

Chlamydospore Germination

 

The ability of seed exudates or their components to stimulate
germination of chlamydospores of E, §91a21_f. sp. pi§i_was determined
using the method of Schroth et a1 (52). Air-dried Conover loam soil
(.5 g) that had been infested with chlamydospores of E, gglagi_f. sp.
pig; (1 x 106 spores/g) was placed in a small petri dish (5 cm diameter),
moistened with 0.2 ml of a test solution, and incubated in a humid con—
tainer for 15 hours at 22°C. The percentage germination was determined
by making a soil smear on a slide, staining it with 0.1% aniline blue in
lactic acid, and counting spores at a.magnification of X 430. One
hundred chlamydospores were counted per slide.

All experiments were repeated at least once with similar re-

sults, except those conducted in the field.

RESULTS

Emergence,_Fresh weight,
and Seed‘Viability

 

 

Bleached, partially bleached, and nonbleached pea seeds were
planted at the Michigan State University Botany Farm on 9 May 1975, in
soil artificially infested with chlamydospores of E, gplapi f. sp. pig},
Seeds were planted 25-30 mm below the soil surface in rows 3.8 meters
long, spaced 60 cm apart. Each treatment was replicated four times,
with 100 seeds per replicate. Seeds coated with 0.8 g thiram.(tetra-
methylthiuram disulfide) (active ingredient) per kg seed served as
controls. All seeds which extended a pumule above the soil surface were
counted as emerged. Emergence of untreated bleached seeds was less than
that of untreated nonbleached seeds, while emergence of partially
bleached seeds was intermediate (Table 2). No significant differences
in emergence were observed between thiram-treated seeds in the field
regardless of bleaching. .All seedlings were a normal green color follow-
ing emergence and appeared normal in growth habit and equal in vigor.

Plants were harvested at maturity by severing vines from the
roots at the soil line, and the fresh weight of the above-ground portion
(leaves, vines, and pods) of the total plant population was determined.
The pods were then shelled mechanically to obtain the fresh weights of
the peas. There were no significant differences in total fresh weights
or shelled pea yields between plants grown from fungicide-treated

bleached or nonbleached seeds. However, plants from untreated

18

19

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omowu oamfluaoavm.omo:oo an zapomofimflowam MoMMAo yo: ow Hoppoa meow may an oozoaaom
cesaoo some :a moon: .COAHwUAHQoa pom mooom OOH .moumUMHmoa 4 mo momozo

.mzou map mofipo>oo ohomon won
mofiuamam poumm “mam .Qm w flqmaom esfiammom mo :ofimqommzm whommooxsmano m coax ooxmymm
who: mooom .ooom mo mx Mom muaofloopmofi o>flpumv.5mhfl:u m w.o u oofloflqumm

 

 

 

 

m me m eNm.H o om venomofim

< 444 m< mem.a m mm emaumoam saamaugaa

< aa4 <.mmm.~ m< mo eonumoanaoz oeauamqsm 02

< Nm4 m< omm.a < ma vasomoam

m< m4m m< mmm.4 m< ma eoauamam sfiamauhma

< 404 m< Nmo.m o< Nw eoauaoageoz oeSUqusm
mmom mood w mood

ooaaocm .mo:m> .mo>moq oocowpoem wowcumoam wuooEumoHH
mmv pcwfloz zmopm compo mo oohwom ooom

 

 

.mwom :oopmmpwz mo oaofix one
.pcmfioz cmopm .ouoowyoeo co pcoaumohp ooom one mqficomofin woom mo mpoommm .N oanmh

20

nonbleached seeds had higher total fresh weights and shelled pea yields
than plants grown from untreated, bleached seeds. When total fresh
weights and shelled pea weights were calculated on a per-plant basis
(Table 3), individual plants from untreated bleached seeds did not
differ significantly in fresh weights or pea yield from untreated non-
bleached seeds, indicating that the plants were similar in vigor once
they were established.

Seeds were germinated in vitro to determine if the differences
in emergence in the field were due to differences in the viability of
bleached, partially bleached, and nonbleached pea seeds. Surface dis-
infested seeds were placed on sterile, moist paper towels for 6 days, at
22°C. The germination rates for all the seeds, regardless of amount of
bleaching, were between 95% and 98%. It was concluded that differences
in emergence between bleached and nonbleached seeds in the field were
not due to differences in seed viability.

Influence of Exudates
onIInfection

 

 

Bleached and nonbleached pea seeds that had been inoculated with
l x 108 conidia per seed of E, splapi_f. sp. pi§1_were leached with
sterile distilled water to remove seed exudates from the host-pathogen
interface. Disease severity was lower for leached seeds of both colors
than for nonleached seeds (Table 4), apparently due to removal of
nutrients exuded. Leached bleached seeds had a higher disease incidence
than leached nonbleached seeds.

It appeared that disease severity could be reduced by continu-
ally removing nutrients from the infection court by leaching the seeds
with distilled water. An experiment was then conducted to determine

whether addition of exudates from bleached or nonbleached seeds to the

21

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an ooonHom nnnflou noeo nfl mneoz .noflueufianon non mooom OOH .mnofiueufiflnoh 4 we mneoz

n
.mzon

 

may mnfipo>oo ouomon won wnfiunefin nopwe amflm .nm .m fineaom enahemnm mo nonnonmnm oponmooxneanu
e nuflz ooxeunm who: mooow .ooom mo mx hon nunofloonmnfl o>fluoev Eenfinu m 0.0 u oofioflmnnme

 

 

 

o on.w o om.m4 om emauemnm

om mm.a om wa.mm mm eeauemnm sanenonea
om< om.e om 40.4m me eoaoeonncoz menonmesm 02

ma mo.m m< 4n.mN we eeaueonm

< no.4 < ma.om ma eogoeonm Annenpnen
m< ma.m Bm< ww.mN mm easemennnoz menonwnsn
meom ooHHonm meom w moon monfl> .mo>eoq oneum Henflmfipo hoHoo epnoeueohe

mwu pnefin nom,»:wao3 swoon mo unoonom ooom ooom

 

 

.mooom eon noopmehflz

oonoeoan no .oonoeoan xaaefippen .oonoeoHnnon thw nzonm muneHm eon Henow>flonfi
wo moaofiz one mpnmfloz :mopm may no unosueopp ooom one wnflnoeofin ooom mo muoommm .m oHoeH

22

Table 4. Effect of leaching with distilled water on infection of
bleached or nonbleached seeds by E, solani f. sp. pisi.

 

 

 

Degree of a Disease Ratingb
Bleaching Inoculated LeachedC Nonleached
Nonbleached yes 0.2 AB 2.1 D
Bleached yes 2.3 D 3.0 E
Nonbleached no 0.1 A 0.3 B
Bleached no 0.0.A 0.7 C

 

3l x 108 conidia/seed.

bo no lesions, 1 = 1-10%, 2 = 11-25%, 3 = 26-50%, 4 = 51-75%,
5 > 75% of the seed was necrotic. Each value is the mean for two
replicates of ten seeds each.

CLeaching dishes (10 seeds/dish) were flushed with 75 m1 of sterile
distilled water every hour. Seeds were incubated for five days at
22°C.

dMeans followed by the same letter do not differ significantly
(P = 0.05) by Duncan's multiple range test.

23
host-pathogen interface would enhance disease expression. Surface
disinfested nonbleached pea seeds (1975) were placed in 25 mm-diameter
test tubes containing 25 g of sterilized l mm—diameter glass beads,
inoculated with 1 ml of a suspension of E, gplgpi_f. sp. pi§i_conidia
(l x 105/ml), and covered with 10 g of sterile glass beads. Then 6 ml of
exudate from nonbleached seeds was added to each tube. Sterile distilled
water served as a control. The tubes were sealed with Parafilm.and in-
cubated for 5 days at 22°C. Inoculated seeds treated with exudate from
bleached seeds had a higher disease incidence than those treated with
exudate from nonbleached seed exudate (Table 5). Disease in inoculated
seeds treated with nonbleached seed exudate did not differ statistically
at P=.05 from that in seedling treated with distilled water, although
disease severity was always higher where exudates were supplied.

An experiment was conducted to determine whether bleached seeds
were more susceptible to E, §91§p1_f. sp. pi§3_than nonbleached seeds
when the inoculum was injected into the cotyledon, thereby eliminating
the influence of seed exudates on disease development. Disease ratings
between bleached and nonbleached seeds did not differ at three inoculum
levels (Table 6). Disease severity increased as inoculum concentration
increased. Therefore, it appears that the greater susceptibility of
bleached seeds to E, gplgpi_f. sp. pi§i_was due to differences in seed
exudation.

Chemical Analysis of
SeedIExudates

 

 

Exudates collected from nonbleached or bleached pea seeds were
analyzed for total water-soluble carbohydrate and ninhydrin-positive
substances to determine if quantitative differences in these components

were associated with the differences in susceptibility expressed by

24

Table 5. Effect of exudates from bleached or nonbleached pea seeds
on infection by E, solani f. sp. 151 of nonbleached pea
seeds in sterile, moist glass beags.

 

 

Treatmenta Disease Rating
Nonbleached Seed Exudate-Inoculatedb 2.1C Ad
Bleached Seed Exudate—Inoculated 3.7 B
Glass Distilled water-Inoculated 1.9 .A
Glass Distilled Water-Noninoculated 0.6 C

 

3Seeds were incubated in exudate solution or glass distilled water
for 5 days at 22°C.

1 x 105 conidia/seed.
C0 = no lesions, 1 = 1-10%, 2 = 11-25%, 3 = 26-50%, 4 = 51-75%,

5 > 75% of the seed was necrotic. Each value is the mean for
two replicates of ten seeds each.

dMeans followed by the same letter do not differ significantly
(P = 0.05) by Duncanfs multiple range test.

25

Table 6. Effect of injection of bleached or nonbleached Miragreen
pea seeds with conidia of E, solani f. sp. pisi.

 

 

 

Treatmenta Disease Ratipgb
Nonbleached Bleached
10 conidia/seed 1.0.AC 0.9 A
100 conidia/seed 1.6 B 1.6 B
1,000 conidia/seed 1.9 B 1.9 B
Distilled water 0.4 C 0.4 C
Noninjected 0.1 C 0.1 C

 

aConidial suspension was injected under the seed coat and the seed was
incubated under sterile, moist conditions for five days, at 22°C.

b0 = no lesions, 1 = 1—10%, 2 = 11-25%, 5 = 26—50%, 4 = 51-75%,

5 - > 75% of the seed was necrotic. Each value is a mean for two
replicates of 10 seeds each.

gMeans followed by the same letter do not differ significantly
(P = 0.05) by Duncan's multiple range test.

26

bleached and nonbleached seeds. Individual sugars and amino acids were
identified from nonbleached and bleached seed exudates to determine if
there were qualitative differences in these components.

Exudates from bleached seeds contained approximately three
times as much total soluble carbohydrate as exudates from nonbleached
seeds (Table 7). Sucrose, glucose, and fructose were identified from
both bleached and nonbleached seed exudates using thin layer chromato-
graphy (Figure 2). These sugars were also identified and quantified
using gas-liquid chromatography (Figure 3, Table 8). All three sugars
were present in larger quantities in bleached seed exudate than in non-
bleached seed exudate. Sucrose was relatively higher in bleached than
in nonbleached seed exudate.

Nonhydrin—positive substances were present at much lower con—
centrations in the seed exudates than were carbohydrates; however, no
significant differences were found in amounts of ninhydrin-positive
substances exuded from bleached or nonbleached pea seeds (Table 7).
Fourteen amino acids were present in the exudates from both bleached and
nonbleached seeds (Table 9). All amino acids identified from the seed
exudates were among those known to be commonly found in proteins. No
significant qualitative or quantitative differences in the amino acid
composition of exudates from nonbleached and bleached pea seeds were

observed.

Chlamydospore Germination

 

Chlamydospores of E, solani f. sp. pisi in natural soil were
used to measure the ability of exudates from bleached and nonbleached
seeds, and some components of these exudates, to stimulate germination

in soil. Cationic, anionic, and neutral fractions of seed exudates, as

27

Table 7. Exudation of carbohydrates and ninhydrinrpositive substances
from pea seeds incubated for 5 days in a moist, sterile,
sand environment at 22°C.

 

 

Degree of ug Carbohydrate pg Ninhydrin-Posit' e
Bleaching per Seeda substances per seed

c d
Bleached 188.37 A. 1.68 C
Nonbleached 68.70 B 1.48 C

 

aCarbohydrate was measured by the anthrone method and is expressed as
glucose equivalents.

bNinhydrin-positive substances is expressed as glycine equivalents.
CEach value is a mean of two replicates of 43 seeds each.

dMeans followed by the same letter do not differ significantly
(P = 0.05) by Duncan's multiple range test.

28

Table 8. Carbohydrates exuded from bleached and nonbleached pea

 

 

 

seeds.
Concentration (nanomoles/seed)a
Carbohydrate Bleaéfied NonBIeaChed
Fructose 102.27 29.94
Glucose 155.72 46.94
Sucrose 184.09 18.02

 

3values represent means of two replicates of 43 seeds each.
Identification and quantification was accomplished using
gas—liquid chromatography.

29

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oouuaoo one nopuouoo o5 ,3 oounooan mpoHoo o5. . Eoeo m: OHV mnemnm oneoneob mo
2:39: .2 one 2w: OHO mnemnm oheoneHm 67m m3: Oev oueonxo ooom oonoeoznn

.N ”Snowy oueonoao ooom oonoeoE .H ”zanwouesonno nob“; 55 e mo nofleunomonnom

 

: o. o o n o n v m N _

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unocuam @
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30

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oonoeoannon Eonm mouepoxnooneo mo mo>fipe>finoo mzH mo monenwouesonnu .omononm .0 one
”moneonepm Henpopnfiv Houflmonfl .m momounam .4 one m mnzonxnn .N momouonhm .H ”one mxeon
.oueonxo ooom eon oonoeoflo Eonm mopepoxnonneu mo mo>ape>flnoo m$:.mo_newmoueeonnu mew

ovw Onu CNN VON om— an. on. OV— U
mm on ON 2 N— a v 0 2:2

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osuods01

 

 

 

 

.m Ban

31

Table 9. Amino acids exuded from bleached and nonbleached pea seeds.

 

Concentration (nanomoles/seed)a

 

 

Amino.Acid Bleached Nonbleached
Aspartic acid 6.22 9.40
Threonine 9.94 8.23
Serine 7.91 13.16
Glutamic acid 8.50 10.52
Glycine 9.28 11.05
Alanine 11.77 15.74
Valine 5.43 7.04
Isoleucine 3.23 4.61
Leucine 6.74 5.74
Phenylalanine 3.92 4.39
Lysine 4.50 3.41
Histidine 4.19 4.35
Arginine 2.33 3.17
Tyrosine 2.75 2.26

 

aValues represent means of two replicates of 43 seeds each.
Identification and quantification was accomplished with an
amino acid analyzer.

32

well as unfractionated exudates, were assayed by applying .2 ml of the
test solution to .5 g of air-dried soil, infested with chlamydospores of
E, §pl§21 f. sp. p1§i_(l x 106 spores/g). Glass-distilled water added
to infested soil served as a control. Spore germination was determined
with soil smears after 15 hours of incubation at 22°C in a humid
environment.

Unfractionated exudate from bleached seeds stimulated more
chlamydospore germination than unfractionated exudate from nonbleached
seeds (Table 10). The neutral (carbohydrate) fraction of bleached seed
exudate also stimulated more chlamydospore germination than did the
neutral fraction of nonbleached seed exudate. Neither the cationic
(amino acid) nor anionic (organic acid) fractions stimulated chlamydo-
spore germination. The unfractionated seed exudates promoted more
chlamydospore germination than did the neutral fractions for both
bleached and nonbleached seeds.

Influence of Sucrose on
Disease Incidence

 

 

Since other experiments had indicated that the carbohydrate
fraction of the seed exudate was influential in the infection process,
the effect of an exogenously applied carbohydrate source on infection
was investigated. Sucrose was chosen as the carbohydrate source to be
tested because it was the predominant sugar component of bleached pea
seed exudate. Surface-sterilized nonbleached pea seeds (1975) were
placed in 25 mm-diameter test tubes containing 25 g of washed silica
sand (sterile), inoculated with 1 ml of a chlamydospore suspension of

E, solani f. sp. pisi (l x 102 chlamydospores/ml), and covered with 10 g

of sterile, washed silica sand. Then 6 m1 of either a 0.1 M sucrose

33

Table 10. Stimulation of E, solani f. sp. pisi chlamydospore
germination in natural soil by bleached or nonbleached
pea seed exudates, or components of these exudates.

 

 

 

Degree of Exudate Chlamydospore
Bleaching Fraction Germination (%)
Nonbleached Unfractionated 16 Ah
Anionic 0 B
Cationic 0 B
Neutral 10 A
Bleached Unfractionated 48 C
Anionic 0 B
Cationic 0 B
Neutral 40 C
Distilled Water - 0 B

 

aValues represent means of two replicates of 100 chlamydospores
each.

bMeans followed by the same letter do not differ significantly
(P = 0.05) by Duncan's multiple range test.

34

solution or distilled water was added aseptically to each tube. The
tubes were sealed and incubated at 22°C for 5 days; the seedlings were
then rated for disease severity. Sucrose~treated seeds had a higher

disease severity than seeds treated with distilled water (Table 11).

35

Table 11. Effect of exogenously applied sucrose on infection of
nonbleached pea seeds by E, solani f. sp. pisi.

 

 

Treatmenta Disease Rating
Sucrose 3.2b AF
Distilled Water 2.1 B

 

3Seeds were incubated in a 0.1 molar sucrose solution for 5 days at
22°C.

b0 = no lesions, 1 = 1-10%, 2 = 11-25%, 3 = 26-50%, 4 = 51-75%,

5 = > 75% of the seed was necrotic. Each value is the mean for

two replicates of ten seeds each.

CMeans followed by the same letter do not differ significantly
(P = 0.05) by Duncan's multiple range test.

DISCUSSION

Bleached pea seeds were found to be more susceptible to
preemergence damping-off than were nonbleached pea seeds under field
conditions. This is in agreement with Short and Lacy (55) who showed
that pea seed and seedling rot was higher among bleached pea seeds than
among nonbleached pea seeds in growth chambers at 20% and 37% soil
moisture. The differences in field emergence could not be explained by
differences in viability of bleached and nonbleached seeds. Macquire
et a1 (29) also reported that bleached and nonbleached seeds of the
wrinkled-seeded cultivar Perfection were equally viable. However,
bleached seeds of the round-seeded cultivar.Alaska were considerably
lower in viability than green seeds.

Total fresh and shelled pea weights of plants grown from non-

bleached seeds were higher than those grown from bleached seeds because
of higher plant populations. However, yields and fresh weights from
individual plants grown from bleached or nonbleached seeds were not
significantly different, suggesting that plants grown from bleached
seeds were similar in vigor to those grown from nonbleached seeds.
This is in contrast to reports that seedlings grown from bleached lima
bean seeds were lower in vigor than those grown from nonbleached seeds
(43, 68).

Qualitative or quantitative differences in pea seed exudates

seemed to be at least partially responsible for the greater

36

37

susceptibility to seed and seedling—infecting fungi of bleached as com-
pared with nonbleached pea seeds. Applications of exudate from bleached
pea seeds to nonbleached seeds increased the susceptibility of these
seeds to infection by E, E91221_f- sp. p3§§_as compared with seeds
treated with nonbleached seed exudate. Flentje (17) showed that wrinkled-
seeded peas were more susceptible to Eythium than smooth-seeded peas
because of differences in seed exudates: smooth—seeded peas planted
below wrinkled-seeded peas, and therefore influenced by the exudate from
the wrinkled-seeded peas, had a higher disease rating than did those
planted below the smooth—seeded peas. In these studies, removing seed
exudates from the host—pathogen interface by leaching with distilled
water did not eliminate the differences in susceptibility between
bleached and nonbleached pea seeds, presumably because the larger amounts
of nutrients exuded by bleached seeds were more difficult to remove.
However, leaching with distilled.water did serve to reduce disease in-
cidence over nonleached controls, suggesting that seed exudates influ-
enced disease incidence or that inoculum.potential was being decreased by
leaching. Bleached and nonbleached pea seeds did not differ in suscepti-
bility when inoculum was introduced into the cotyledons of the seed,
thereby eliminating the influence of seed exudates. Beute (7) showed
that the increase in Fusarium root rot of virus-infected pea plants was
due to an increase in root exudation by injecting spores of E. M}; f.
p;§}_into the cortical tissues of the stems of pea plants: lesions
produced on healthy and virus—infected plants were equal in severity.

The quantity of carbohydrate exuded from pea seeds was correla-
ted with susceptibility of pea seeds to preemergence mortality. Approxi-
mately three times more carbohydrate was present in the exudate from

bleached seeds than in exudates from nonbleached seeds. This confirmed

38
work by Short and Lacy (54) and Maquire et a1 (29) showing carbohydrate
exudation to be 3-5 times higher from bleached than from nonbleached pea
seeds. There were no quantitative differences in ninhydrin-positive sub-
stances and no qualitative differences in sugars or amino acids in
exudates from nonbleached or bleached pea seeds. Since optimal germina—
tion of chlamydospores of Fusarium.in soil can be achieved with several
sugars or nitrogen sources (14), stimulation of disease by specific
sugars or amino acids was not expected. Similar arrays of sugars and
amino acids have been reported to occur in exudates from other seeds:
all three sugars and 10 of the amino acids were found in pine seed
exudates (3), while the three sugars and amino acids were identified from
exudates of cotton (19) and bean (52) seeds.

Chlamydospores of E, gplgpi f. sp. pi§1_germinated only in
response to the carbohydrate fractions of both bleached and nonbleached
seed exudates, showing that the carbohydrate component of the seed
exudate was primarily responsible for stimulating chlamydospores of E,
§21§22.f- sp. pig; to germinate in the spermosphere of pea. Higher
chlamydospore germination in response to the carbohydrate fraction of
exudates from bleached pea seeds than from nonbleached pea seeds re-
flected higher amounts of carbohydrate in exudates from bleached seeds.
Cook and Schroth (14) have shown that a reduced amount of available
carbon was the principle factor limiting germination of chlamydospores
of Fusarium in soil. Unfractionated pea seed exudate was more stimula-
tory to germination than was the carbohydrate fraction, suggesting that
other components of the exudate serve to enhance germination. It is
possible that nitrogen was somewhat limiting to germination when only
the carbohydrate fraction was supplied. Germination of chlamydospores

of Fusarium in soil was higher when both amino acids and sugars were

39

supplied than when only simple sugars were added (14). Amino acids are
sources of both carbon and nitrogen, and thus have the ability to
stimulate germination of chlamydospores (3, 15, 50, 52). The fact that
the amino acid fraction of the seed exudates did not stimulate chlamydo—
spore germination.may have been because the quantity of amino acids
present was not high enough to fulfill the energy requirements for
chlamydospore germination in soil.

Increased disease severity in response to the addition of
sucrose to the host—pathogen interface suggested that the high carbohy-
drate exudation from bleached seeds could be responsible for increased
pre-emergence damping—off in the field. Keeling (25) found that there
was a direct relationship between the amount of preemergence seed and
seedling rot of soybean caused by Eythium, and the amount of carbohy—
drates exuded by germinating seeds: more than twice the quantity of
carbohydrate was exuded from seeds of a susceptible cultivar than from
a resistant cultivar. Similar correlations of carbohydrate exudation
and seed and seedling susceptibility to soil—borne pathogens have been
made in other studies (17, 26, 33).

Carbohydrate exuded from seeds or roots serve to stimulate
spore germination and increase the inoculum potential of the pathogen
in the spermosphere or rhizosphere, resulting in increased disease
incidence (49). Exudation of carbohydrate would be expected to in-
crease the rate of spore germination and inoculum potential until other
factors, such as nitrogen, become limiting to the fungus. However, the
stimulation of the pathogen in the spermosphere or rhizosphere by host
exudates is affected by the activities of other microorganisms which

occupy the same microhabitat as the pathogen, and therefore influence

40

both its saprophytic and pathogenic activities (49). In certain circum-
stances, exudation may favor antagonistic microorganisms more than the
pathogen, the net effect being a reduction in disease severity: a
number of reports have indicated the importance of antagonists in
suppressing the growth of Fusarium (9, 35, 36, 37, 41).

The effect of seed and seedling exudation on disease incidence
depends to a large extent on the nature of the exudates. Exudation of
nutrients from seeds and roots is dramatically influenced by environ-
mental parameters, such as soil moisture (24, 26), high (20) and low
(22) temperatures, and anaerobic conditions (8), as well as by the
collection method used (5). Present methods of exudate collection and
analysis do not permit quantification of the concentration of nutrients
at the host-pathogen interface under natural conditions. The develop-
ment of techniques to measure nutrient concentrations in the soil would

greatly increase the significance of plant exudate analysis.

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10.

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