New record of Phytophthora root and stem rot  
of Lavendula angustifolia 

LESZEK B.ORLIKOWSKI1 and ALMA VALJUSKAITE2

1Research Institute of Pomology and Floriculture 
Pomologiczna 18, PL-96-100 Skierniewice, lorlikow@insad.pl 

2Lithuanian Institute of Horticulture, Plant Protection Laboratory 
Babtai, Kauno 30, LT-54333

O r l i k o w s k i  L.B., Va l j u s k a i t e  A.: New record of Phytophthora root and stem rot of 
Lavendula angustifolia. Acta Mycol. 42 (2):193-198, 2007.

Phytophthora cinnamomi was isolated from rotted root and stem parts of lavender as well 
as from soil taken from containers with diseased plants. Additionally Botrytis cinerea, Fusarium 
spp. and Sclerotinia sclerotiorum were often isolated from diseased tissues. P. cinnamomi 
colonised leaves and stem parts of 4 lavender species in laboratory trials and caused stem rot 
of plants in greenhouse experiments. Cardinal temperature for in vitro growth were about 7,5 
and 32°C with optimum 25-27,5°C. The species colonised stem tissues at temperature ranged 
from 10° to 32°C.

Key words: stem rot, isolation, Phytophthora cinnamomi, colonisation, temperature, growth

INTRODUCTION

Lavender (Lavendula angustifolia Mill., syn. L.officinalis Chaix) is main-
ly medicinal and pharmaceutic plant but since the last years it has been grown 
in ornamental nurseries mainly as small, blooming, hedge culture. The quality 
of plants may be strongly decreased by Phytophthora species. From diseased 
plants mainly Phytophthora nicotianae var. parasitica was isolated (P a p p a s 
1978; P u t m a n  1991; M i n u t o  et al. 2001a). Growing of plants in Italy un-
der shade and in larger pots reduced disease incidence caused by that species  
(M i n u t o  et al. 2001a). Variable results were obtained with susceptibility of cultivars or 
local selections toward the pathogen (M i n u t o  et al. 2001b). P a e z  et al. (1993) recovered  
P. palmivora Butler from diseased Lavendula dentata grown in Spanish gardens whereas  
D a v i n o  et al. (2002) isolated the species from rotted root of L. angustifolia in 
Italy.

In 2003 on lavender mother plants grown on greenhouse beds yellowing and 
browning of single shoots were observed. The disease spread slowly on neighbouring 

 ACTA MYCOLOGICA
 Vol. 42 (2): 193-198
 2007

Dedicated to Professor Alina Skirgiełło 
on the occasion of her ninety-fifth birthday



194 L.B. Orlikowski and A. Valjuskaite 

shoots. After the next 6 weeks 3/4 parts of affected plants were destroyed (Fig.1). 
On mother plants dark-gray spots on the shoot bases, browning during the next few 
days and spreading on roots, upwards and on the periphery of affected stems were 
observed. The disease spread quickly on neighbouring mother plants and cuttings. 
On plants growing in container - grown nursery brown or dark-brown spots devel-
oped on individual shoots spread on roots and upwards. During the next 10 days 
single or a few yellow-brown to dark-brown shoots on individual plants were seen. 
The development of symptoms were observed during 2 years before or during flow-
ering of plants. The objective of this investigation was to determine a causal agent of 
lavender shoot and root rot, development of disease in laboratory and greenhouse 
trials and relationship between temperature and growth of Phytophthora cinnamomi 
and colonisation of stem parts of plants.

MATERIALS AND METHODS

Survey of lavender in greenhouse and container - grown nursery. On plants 
grown in greenhouse shoot rot symptoms were observed only in one year on about 
5% of lavender. In container - grown nursery lavender were grown at least 10 years 
but shoot and root rot symptoms occurred in years 2004 and 2005 on about 10 and 
20%,respectively. Diseased plants were collected in plastic bags and transferred to 
laboratory. The next day plants were removed from pots, substratum were collected 
in bags whereas plants were washed under tap water and affected shoots were sepa-
rated, rinsed 3times in distilled water, blotting dried and chosen parts were sterilised 
over a burner flame. About 5 mm long stem parts were put on PDA medium and 
plates were checked during 4-day-incubation at 24°C in the dark on the presence of 
Phytophthora and other genera. Additionally, substratum samples, taken from pots 
with lavender showing disease symptoms in greenhouse and nursery, were analysed 
on the presence of Phytophthora spp. in years 2003-2005. Substratum taken from 3-6 
pots was mixed about 5 min in plastic bag and half liter of it was put into plastic box, 
flooded with tap water (about 1 l) and rhododendron leaves cv. Zembla were floated 
over flooded sample (16 leaf blades/box). Boxes covered with plastic foil were incu-
bated at temperature 22-24°C. After 4-6-day-incubation leaves with necrotic spots 
were removed, washed with distilled water, blotted dried, disinfected over a burner 
flame and about 5 mm diameter plugs were transferred on PDA medium. Small parts 
of colonies, grown around tissues were transferred to PDA slants. Cultures from dis-
eased stems and substratum were grouped on the base of their growth and morpholo-
gy and chosen, representative isolates were identified to genera and species (S z k u t a 
2004). Confirmation of Phytophthora classification to species was performed by DNA 
analyses using the method described by O r l i k o w s k i  et al. (2006).

Colonisation of lavender by Phytophthora cinnamomi. In laboratory trials leaves 
and stem parts of 4 cultivars of lavender (Tab. 1) were put into plastic boxes on 
sterilised, wet blotting paper covered with plastic net and inoculated with 3mm plugs 
taken from the edge of 5-day-old cultures of P. cinnamomi (2 isolates from diseased 
stem base and substratum) growing on PDA at 24°C in the dark. Boxes were covered 
with foil and incubated at 22-24°C in the dark. After 5-day-incubation diameter and 
length of necrosis was measured. In greenhouse trial stem bases of 3 cultivars of lav-
ender were inoculated with 3 mm diam plugs of P. cinnamomi (from diseased stem 



 New record of Phytophthora 195

base) and incubated under covering 12 days. Length of necrosis was measured 8 and 
12 days after inoculation.

Relationship between temperature, ranged from 7,5 to 35°C, growth of P. cin-
namomi and colonisation of lavender stem parts by the species were studied using 
the same procedure like in laboratory trials.

Experimental design was completely randomised with 4 replications and 10 
leaves, stem parts or plants in each rep. Growth of the species on PDA was esti-
mated on the base of 5 Petri dishes for each temperature. Trials were repeated at 
least twice.

RESULTS AND DISCUSSION

Isolation of fungi and Algae-like Oomycetes. Similar genera and species were iso-
lated from plants taken from greenhouse and field production (Tab. 2). From potential 

Ta b l e  1 
Phytophthora cinnamomi isolated from substratum used for lavender growth; mean number 

of dark-brown spots on rhododendron leaves used as the bait

Source of substratum Year of analysis
2003 2004 2005

Greenhouse 25.5 b - -
Container nursery 14.0 a 10.8 a 17.6 ab

Note: Means followed by the same letter do not differ with 5% of significance (Duncan’s multiple range 
test)

Ta b l e  2 
Fungi and Algae-like Oomycetes isolated from diseased base of Lavendula angustifolia; 

number of settled plants (a) and number of isolates obtained (b)

Genera/species Year of isolation
2003

greenhouse  
(27 plants)

2004
field (14 plants)

2005
field (21 plants)

a b a b a b
Alternaria alternata Nees 2 5 6 11 8 13
Botrytis cinerea Pers. 7 11 4 9 5 11
Cladosporium herbarum (Pers.) Link. 3 3 - - 2 4
Fusarium culmorum (W.G.Sm.) Sacc. 4 7 2 5 - -
Fusarium equiseti (Cda) Sacc. 3 5 - - 3 7
Fusarium solani (Mart.) Sny. et Hans. 6 7 3 5 1 3
Humicola grisea Traaen 1 2 - - 2 5
Mucor spp. 4 8 5 9 7 16
Penicillium spp. 3 5 2 4 - -
Phytophthora cinnamomi Rands 18 56 9 29 18 44
Rhizopus sp. - - 2 4 - -
Sclerotinia sclerotiorum (Lib.) de Bary 4 10 - - 2 7
Trichoderma spp. 3 6 3 7 4 7



196 L.B. Orlikowski and A. Valjuskaite 

pathogens of lavender Botrytis cinerea (mainly in field), two Fusarium species, Phytoph-
thora cinnamomi and Sclerotinia sclerotiorum were detected from diseased plant parts.  
P. cinnamomi (Fig.2) was the most often isolated species both, in greenhouse and 
field - grown plants. The species was detected from 3/4, 5/7 and 6/7 of analysed 
plants, respectively (Tab. 2).

Isolation of Phytophthora cinnamomi from substratum. Using rhododendron 
leaves as the bait, P. cinnamomi was detected from substratum samples taken from 
60 pots with plants showing Phytophthora rot symptoms. Significantly more necrotic 
spots were observed on rhododendron leaves floated in suspension of substratum 
collected from diseased lavender grown in greenhouse (Tab. 1).

Colonisation of lavender by Phytophthora cinnamomi. Both isolates of  
P. cinnamomi used for lavender inoculation in laboratory trials, caused necrosis of 
leaves and stem parts of 4 tested cultivars (Tab. 3). On stem parts necrosis spread 
faster than on leaves. In case of leaf blades inoculation, isolate from substratum 
colonised tissue slower than that from the stem base. On leaves of cv. Grosso necro-
sis spread at least 1/3 faster than on 3 other cultivars. On stem parts such differences 
were not observed (Tab. 3).

Ta b l e  3 
Colonisation of leaves and stem parts of lavender by Phytophthora cinnamomi; diam/length 

(in mm) of necrosis after 5-day-incubation 
Inoculation: 2005.09.27

Source of P. cinnamomi Cultivars Leaves Stem parts
Base of stem Blue Dafo 32.3 ab 43.3 a

Edelweiss 35.0 bc 40.3 a
Grosso 32.0 a 39.5 a

Munstead 35.5 c 38.8 a
Substratum Blue Dafo 19.5 b 46.3 b

Edelweiss 15.3 a 38.8 a
Grosso 30.8 c 45.3 ab

Munstead 22.5 b 38.3 a

Note: Means in columns followed by the same letter do not differ with 5% of significance; 
means separation for the source of the species

Ta b l e  4 
Spread of necrosis (in mm) on lavender stems inoculated with Phytophthora cinnamomi 

from the stem base in relation to cultivars and incubation time; greenhouse trials 
Inoculation: 2005.11 17

Cultivars Length of necrosis in mm after days of incubation
8 12

Blue Dafo 66.5 b 87.6 b
Grosso 53.4 a 73.7 ab

Munstead 48.7 a 65.3 a

Note: see Table 3





198 L.B. Orlikowski and A. Valjuskaite 

SUMMARY

The objective of this investigation was to determine a causal agent of lavender 
shoot and root rot, development of disease on plant parts and relationship between 
temperature and growth of pathogen and disease development. During 3 years my-
cological analyse of diseased lavender, taken from greenhouse and container nurs-
ery, was done. Additionally, the presence of P. cinnamomi in substratum was esti-
mated using rhododendron leaves as the bait. Phytophthora cinnamomi was isolated 
from the most of analysed plants and from substratum. Botrytis cinerea, Fusarium 
spp. and Sclerotinia sclerotiorum as other potential pathogens, were recovered from 
diseased shoot parts. Isolates of P. cinnamomi from plant and substratum colonised 
lavender leaves and stem parts of all tested cultivars. In greenhouse experiment the 
species quickly colonised stem tissues and necrosis spread about 5,6 mm/24 hr. The 
growth of the pathogen on PDA and colonisation of stem parts were observed at 
temperature range from about 7,5 to 32,5 °C with optimum 25 -27,5°C.

REFERENCES

D a v i n o  S., C a c c i o l a  S. O., P e n n i s i  A. M., D e s t r i  N i c o s i a  M. G. 2002. Phytophthora palmivora 
a new pathogen of lavender in Italy. Plant Disease 86 (5): 561.

M i n u t o  A., G u l l i n o  M. L., T i t o n e  P., G a r i b a l d i  A. 2001. Influence of cultural practices on inci-
dence of Phytophthora nicotianae var. parasitica causing root rot of lavender (Lavendula officinalis 
L.). Phytopathol. Meditterranea 40 (1): 45–54.

M i n u t o  G., A r m a t o  B., G i l a r d i  G., G a r i b a l d i  A. 2001. First observations on susceptibility of 
Lavendula spp. to Phytophthora nicotianae var. parasitica. Informatore Fitopatologico 51 (5):69–72.

O r l i k o w s k i  L.B., Tr z e w i k  A., W i e j a c h a  K. 2006. Phytophthora tropicalis, a new pathogen of orna-
mental plants in Poland. J. Plant Prot. Res. (in print).

P a e z  J. I., B e r r a  D., Ve g a  J. M., Te l l o  J. 1993. Identification de Phytophthora palmivora Butler en 
jardines de la Exposicion Universal de Sevilla. Bol. de Sanidaad Vegetal, Plagas 19 (4): 633–447.

P a p p a s  A. 1978. New diseases caused by Phytophthora spp. Phytophthora Newsl. 6: 72–73.
P u t n a m  M. 1991. Root rot of lavender caused by Phytophthora nicotianae. Plant Pathol. 40: 480–482.

Występowanie zgnilizny korzeni i pędów,  
powodowanej przez Phytophthora cinnamomi, na Lavendula angustifolia 

S t r e s z c z e n i e

Celem badań było określenie przyczyny zgnilizny pędów i korzeni lawendy, rozwo-
ju choroby w doświadczeniach laboratoryjnych i szklarniowych oraz współzależności po-
między temperaturą a wzrostem in vitro patogena oraz kolonizacją części łodyg. W ciągu 
3 lat prowadzono analizę mikologiczną chorych roślin lawendy, pobieranych ze szklarni 
oraz ze szkółki pojemnikowej. Dodatkowo, stosując pułapki z liści różanecznika izolowa-
no Phytophthora spp. z podłoża. Z większości chorych roślin, a także z podłoża izolowano 
Phytophthora cinnamomi. Z innych organizmów izolowano Botrytis cinerea, Fusarium spp.  
i Sclerotinia sclerotiorum. Izolaty P. cinnamomi z porażonej rośliny i podłoża kolonizowały 
liście i części łodyg wszystkich badanych odmian lawendy. W doświadczeniu szklarniowym 
omawiany gatunek szybko kolonizował tkanki pędów, a nekroza rozwijała się ok. 5,6 mm/
dobę. Wzrost P. cinnamomi na pożywce PDA oraz kolonizację pędów obserwowano w tempe-
raturze od 7,5° do 32,5°C z optimum 25-27,5°C. 



Fig. 2. Zoosporangia of Phytophthora cinnamomi and released zoospores. Phot. G. Szkuta.

Fig.1. Phytophthora shoot and stem rot of lavender cuttings. Phot. L. B. Orlikowski.


		2014-01-01T11:46:10+0100
	Polish Botanical Society