Annual Report 2020

Page 87

Outlook We are constantly working to optimize the real-time PCR method. This involves continuously verifiying that the primers used in the PCR reaction for the detection of Verticillium nonalfalfae can still detect all mild and aggressive versions that occur in the Hallertau.

References Borza, T., Beaton, B., Govindarajan, A., Gau, X., Liu, Y., Ganga, Z., Wang-Pruski, G. (2018): Incidence and abundance of Verticillium dahliae in soil from various agricultural fields in Prince Edward Island, Canada. Eur J Plant Pathol 151, 2825—2830. https://doi.orgll 0.1007/310658—017—1408-1 EPPO Bulletin (2020) PM 7/78 (2) Verticillium nonalfalfae and V. dahliae: 50 (3): 462-476. Guček, T., Stajner, N., Radišek, S. (2015): Quantification and detection of Verticillium albo-atrum in hop (Humulus lupulus) with real-time PCR. Hop Bulletin 22, 26-39. Maurer, K.A., Radišek, S., Berg, G., Seefelder, S. (2013): Real-time PCR assay to detect Verticillium albo-atrum and V. dahliae in hops: development and comparison with a standard PCR method. Journal of Plant Diseases and Protection, 120 (3), 105–114. Seigner, E, Haugg, B, Hager, P., Enders, R., Kneidl, J. & Lutz, A. (2017): Verticillium wilt on hops: Real-time PCR and meristem culture – essential tools to produce healthy planting material. Proceeding of the ScientificTechnical Commission of the International Hop Growers´ Convention, Austria, 20-23. Wei, F., Fan, R., Dong, H.-T., Shang, W.-J., Xu, X.-M., Zhu, H.-Q., Yang, J.-R., and Hu, X.-P. (2015): Threshold microsclerotial inoculum for cotton Verticillium wilt determined through wet-sieving and real-time quantitative PCR. Phytopathology 105:220-229. Weller, S.A., Elphinstone, J.G., Smith, N.C., Boonham, N., and Stead, D.E. (2000): Detection of Ralstonia solanacearum strains with a quantitative, multiplex, real-time, fluorogenic PCR (TaqMan) assay. Appl Environ Microbiol. 66(7), 2853-8.

6.8

Meristem culture for the production of healthy seedlings

Project Management: Team: Collaboration:

Dr. E. Seigner, A. Lutz B. Haugg P. Hager, R. Enders, IPZ 5c Dr. L. Seigner, and the Virus Diagnostics Team, IPS 2c

Objectives Infestations of Verticillium, viruses, and viroids can lead to dramatic losses in yield and quality. Since these diseases cannot be combated with pesticides, a biotechnological method, such as meristem culture, is used to produce Verticillium- and virus-free material. In 2020, the main focus was on improving the method for eliminating apple mosaic virus (ApMV), which is often more stubborn than the hop mosaic virus and can still be detected in regenerated plants, even after a meristem culture intervention.

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6.8 Meristem culture for the production of healthy seedlings

6min
pages 87-90

detection of Verticillium directly in the bine using real-time polymerase chain reaction (PCR

13min
pages 81-86

Pseudoperonospora humuli

6min
pages 77-80

7.2.2 Alternative uses of hops

3min
pages 100-101

6.5 Powdery mildew isolates and their use in breeding of mildew resistant hops

5min
pages 74-76

content and particular suitability for cultivation in the Elbe-Saale region

8min
pages 69-73

5.6 CBCVd-Monitoring 2020

2min
pages 61-62

5.1.2 Arrival of aphids in 2020

0
page 53

5.2 GEP Quality Audits

0
page 54

6.3 Crossbreeding with the Tettnanger landrace

7min
pages 66-68

5.5 GfH-Project in Verticillium Research

10min
pages 56-60

fertigation

4min
pages 44-46

of irrigation and the position of the drip hose

4min
pages 37-39

fertilizer systems (ID 6054

2min
pages 32-33

1.2 Harvest volumes, yields, and alpha acid contents

4min
pages 12-15

nitrogen fertilization

6min
pages 40-43

optimize the nutrient efficiency of organically bound nitrogen (ID 6141

4min
pages 34-36

3.5 IPZ 5e – Ecological issues in hop cultivation

1min
page 24

3.2 IPZ 5b - Crop protection in hop production

1min
page 20

systems with fertigation (ID 5612

8min
pages 27-31
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