10/20/2021
Introduction to Biopharmaceutical Manufacturing October 20‐22, 2021
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Instructors
Beth Zielinski‐Habershaw, Ph.D., PDI, The University of Rhode Island Sharon McGuire, MS, PDI, The University of Rhode Island Cahil McGovern, Ph.D., PDI, The University of Rhode Island Malcolm Pluskal, Ph.D., Landrau Scientific Innovations
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Day 1
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Industry Status Update 2021
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2018 was a record year for new drug approvals FDA Expedited Pathways and Other Approval Attributes 2017 and 2018 Designation or Attribute
2017 (N = 46)
2018 (N = 59)
Orphan Designation
18 (39%)
34 (58%)
Fast Track Designation
18 (39%)
24 (41%)
Breakthrough Therapy Designation
17 (38%)
14 (24%)
Priority Review
28 (61%)
43 (73%)
Accelerated Approval
6 (13%)
4 (7%)
First‐Cycle Approval
39 (85%)
56 (95%)
First Approved in US
36 (78%)
42 (71%) Source: https://www.raps.org
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What about 2020?
Source: fda.gov/news‐events Source: https://www.raps.org
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Registered Studies as of February 4, 2020 ClinicalTrials.gov currently lists 329,173 studies with locations in all 50 States and in 209 countries
Location
Number of Registered Studies and Percentage of Total (as of February 4, 2020)
Non‐U.S. only
161,669 (49%)
U.S. only
111,377 (34%)
Both U.S. and non‐U.S.
17,133 (5%)
Not provided
38,994 (12%)
Total
329,173 (100%) Source: https://clinicaltrials.gov
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Registered Studies as of February 4, 2021 ClinicalTrials.gov currently lists 364,943 studies with locations in all 50 States and in 209 countries
Location
Number of Registered Studies and Percentage of Total (as of January 24, 2021)
Non‐U.S. only
183,505 (50%)
U.S. only
120,000 (33%)
Both U.S. and non‐U.S.
18,754 (5%)
Not provided
42,864 (12%)
Total
364,943 (100%) Source: https://clinicaltrials.gov
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Clinical Studies include: Biologicals New molecular identities Small molecules Cell Therapy* Gene Therapy* Medical Devices Combination products Biosimilars
Intense Efforts
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Along with the Biologicals, things to watch on the horizon…. CART Cell Therapies…. Chimeric antigen receptor T cells are T cells that have been genetically engineered to produce an artificial T‐cell receptor for use in immunotherapy. Kymriah CAR‐T therapy (Novartis): $475,000 Yescarta CAR‐T therapy (Gilead): $373,000
Developmental areas: logistics: cryopreservation and thawing
Autologous vs. Allogeneic (treating individuals vs. treating populations) Forecast Can anticipate 50 new cell therapy approvals in the next 2‐3 years
Cell therapies‐ others
Blood vessels Skin 3D printed organs Vaccines
Source: https://weillcornell.org/
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Autologous vs. Allogeneic Therapies Autologous (treating individuals‐the starting material and finished product are the same cells) Immunogenic benefits Patient variability Small scale manufacturing lots
Allogeneic (treating populations) Less complex in nature‐use of characterized cell banks Potential immunogenicity Potential tumor formation
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Autologous Manufacturing Process Source: BioProcess International April, 2019 page 16
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Gene Therapy…. Gene Therapies…. Replacing faulty genes with the corrected version using viral delivery systems Luxturna (Spark): $425,000 (per eye) Zolgensma (Novartis): $2,100,000 LentiGlobin/Zynteglo (Bluebird): $1,800,000
Candidates in development include: Hemophilia (Phase 3‐Spark/Pfizer) ALS (Phase 1‐ALS Association) Retinitis Pigmentosa (SKYLINE; Phase 2)
Source: http://www.alsa.org/
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Pharmaceutical Products vs. Biological Products Pharmaceutical Products are more commonly known as medicines or drugs which are chemically produced and have low molecular weights. Typically, these have simpler structures. Biological Products are more complex products which typically are produced through living systems, such as microorganism, plant cells, or animal cells and are often more difficult to characterize than traditional pharmaceuticals. These also have high molecular weights and have complex structures (primary through tertiary structures).
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Pharmaceutical Products vs. Biological Products
Source: https://www.google.com/search?q=small+chemical+molecule+vs+complex+biologic
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Example: Ibuprofen vs. CNTF Ibuprofen (C13H18O2)
anti‐inflammatory molecular mass of about 206 Da
CNTF (C1018H1598N288O298S5)
neuroprotective molecule approximately 200 amino acids molecular weight of 23,000 Da (relatively small compared antibodies which are in the 100‐150 KDa range, bifunctional antibodies are even larger (500 KDa)).
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Example: Ibuprofen vs. CNTF
Ibuprofen
Source: https://www.researchgate.net/
CNTF Source: https://en.wikipedia.org/
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Top 200 Brand‐ Name Drugs by Retail Dollars 2006 Source: https://njardarson.lab.arizona.edu Njardarson Group
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Top 200 Pharmaceutical Products by Retails Sales in 2018 Source: https://njardarson.lab.arizona.edu Njardarson Group
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Top 200 Pharmaceutical Products by Retails Sales in 2019 Source: pharmaexcipients.com
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Top 10 Biologicals (updated June 23, 2020) Name
Manufacturer AbbVie
Launch Date 2001
Global Sales $18.4B
Humira
Rituxan
Roche
1997
$9.2B
Enbrel
Amgen/Pfizer
1998
$7.9B
Herceptin Avastin
Roche Roche
1998 2004
$7.4B $7.1
Remicade
J&J/Merck
1998
$7.1
Lantus Neulasta Avonex Lucentis
Sanofi Amgen Biogen Roche/Novartis
2000 2002 1996 2006
$5.7 $4.7 $2.1B $5.1B
Indications Rheumatoid arthritis, plaque psoriasis, Crohn’s disease, ulcerative colitis, ankylosing spondylitis, psoriatic arthritis, polyarticular juvenile idiopathic arthritis Non‐Hodgkins lymphoma, chronic lymphocytic leukemia, rheumatoid arthritis Rheumatoid arthritis, plaque psoriasis, psoriatic arthritis HER2+ breast cancer Breast, colorectal, kidney, non‐small‐cell lung, glioblastoma, ovarian cancers Rheumatoid arthritis, Crohn’s disease, ankylosing spondylitis, psoriatic arthritis, plaque psoriasis, ulcerative colitis Diabetes Neutropenia related to cancer chemotherapy Multiple sclerosis (MS) Age‐related macular degeneration Source: verywellhealth.com
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Biosimilars (are not generics) Biosimilars (also known as follow‐on biologic or subsequent entry biologic) is a biologic medical product that is almost an identical copy of an original product that is manufactured by a different company. Biosimilar approvals have stalled (somewhat) despite 22 approvals (as of October 2019). Not anymore (February 2021) In the US 26 are approved/17 on the market Sales expected to triple ($2.4B to $6.5B)
Zarxio Amjevita Ixifi
Neupogen Humira Remicade
Source: https://www.zarxio.com/biosimilars
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Bi‐Specific Antibodies Large molecule Fusion protein Two separate and distinct variable regions Can be cellularly produced AMG 420 Myeloma and T cell binder
Manufacturing hurdles (can be overcome) Source: https://www.amgenscience.com/
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Bi‐Specific Antibodies Under Investigation
Source: Amgen’s BITE Engager, 2020
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Other Trends to watch for....... Combination Products (combination of device and cells or slow release biologicals) Biodegradables Slow releasing polymers
Living implants Artificial organs Encapsulated cell implants 3D printed organs/bioprinting
Reservoirs (delivery systems)
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Let’s begin……
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Therapeutic Gene R&D and Product Development
Typical Biological Manufacturing Process Flow Diagram (Mab)
Expression Vector / Host Cell Line Development
ICH Q5A Q5B Q5D Q6E
Clone
Research Cell Bank (RCB) Cell Banking
Upstream Manufacturing
Q7
Master Cell Bank (MCB) Working Cell Bank (WCB)
USP Drug Substance Cell Culture Scale‐up N‐2, N‐1, N
Cell Culture / Seed Train / Bioreactor
Downstream Manufacturing
Harvest / Clarification
Q7
ICH Q5A Q5C Q5E Q6B Q11
• • • • • •
Purification Capture Viral Inactivation UF / DF Polish Viral Filtration UF / DF
Bulk Drug Substance Formulation & Fill
Clarified Bulk
ICH=International Conference on Harmonization Guidance USP=United States Pharmacopeia A typical biologic manufacturing process flow diagram with appropriate ICH guidance steps. (Source: Cytovance Biologics Inc. John Conner, 2013.)
DSP Process Drug Product
Drug Product Formulation & Sterile Formulation & Fill
Q5E, Q6B, Q8
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Therapeutic Gene R&D and Product Development
Typical Biological Manufacturing Process Flow Diagram (Mab)
Expression Vector / Host Cell Line Development
ICH Q5A Q5B Q5D Q6E
Clone
Research Cell Bank (RCB) Cell Banking
Upstream Manufacturing
Q7
Master Cell Bank (MCB) Working Cell Bank (WCB)
USP Drug Substance Cell Culture Scale‐up N‐2, N‐1, N
Cell Culture / Seed Train / Bioreactor
Harvest / Clarification
Downstream Manufacturing
YOU! Q7
ICH Q5A Q5C Q5E Q6B Q11
• • • • • •
Purification Capture Viral Inactivation UF / DF Polish Viral Filtration UF / DF
Bulk Drug Substance Formulation & Fill
Clarified Bulk
ICH=International Conference on Harmonization Guidance USP=United States Pharmacopeia A typical biologic manufacturing process flow diagram with appropriate ICH guidance steps. (Source: Cytovance Biologics Inc. John Conner, 2013.)
DSP Process Drug Product
Drug Product Formulation & Sterile Formulation & Fill
Q5E, Q6B, Q8
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Identifying Potential Therapeutic Molecules
You have a target and let’s say that it is known to cause inflammation You have a known mechanism of action A
Inflammation
A
No Inflammation B
You have the sequence of a protein that you know binds to protein A in such a way that it interferes with the mechanism of action You know both the protein sequence and genetic (DNA) sequence So you want to make lots of your molecule but to get there, a few steps are needed……
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Monoclonal Antibodies Common production molecules High specificity (low occurrence of cross reactivity) Lock and key mechanism
Can be easily expressed in cell lines Favorable half life (compared to other molecules)
Source: https://en.wikipedia.org/
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Wait……… First, everyone needs to realize that biomanufacturing is 100% a team sport. What you do has a ripple effect….. You rely on the people upstream from you (R&D, PD, etc.) to do their job. Likewise, the people downstream from you (clinicians, patients, etc.) rely on you to do your job.
Most important Source: https://www.nepatriots.com
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Vector Design and Creation of Cell Lines Objective: create a vector that can be used to stably transfect a cell line which has the quality attributes of genotypic and phenotypic stability 32
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Step 1: Vector Design Characteristics of plasmids
Selection markers (vary) Amplification strategy Polyadenylation signals MARS sequences Multiple cloning sites (MCS) ECO RI Bam HI
Source: https://www.invivogen.com/pcpgfree
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Gene Amplification Genes can be amplified once they have been incorporated into the cell pCpG free plasmids Decreased methylation MARS sequences
DHFR/Methotrexate (or GS/MSX system) Found in plasmids like pNUT Methotrexate
Targets DHFR (dihydrofolate reductase) an enzyme that is essential for thymidylate biosynthesis Glycine synthesis Inhibits purine and pyrimidine synthesis (plays an important role in DNA and RNA synthesis) Placing the gene of interest close to DHFR and culturing cells in increasing amount of MTX followed by selection.
Source: https://www.albert.io/blog/g1‐g2‐phases‐cell‐cycle
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How does this happen? TargetGene Antibody B Genetic code
Cut open (digest) plasmid using enzymes for the target gene (creating sticky ends) Ligate plasmid and target gene Transform bacteria and grow up the plasmid
Source: https://www.khanacademy.org
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Step 2: Identifying Your Workhorse Cell Line Mammalian Cells Insect Cells Yeast Bacteria Mammalian cells (adherent CHO‐K1)
Bacteria Source: https://www.phe‐culturecollections.org.uk Source: https://www.researchgate.net Source: https://www.quora.com
Yeast 36
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Why use CHO cells? Advantages
Easy to manipulate genetically Adaptable to serum/protein free media Large‐scale suspension culture Insusceptible to human pathogens Capable of human like glycosylation
Disadvantages Genomic/phenotypic instability Potential decreases in productivity
Suspension CHO cells https://www.ncbi.nlm.nih.gov/books/NBK100915/figure/ionchannel.F14/
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Methods of Transfection Methods
Microinjection Gene gun Electroporation Viral transduction Lipofection
Source: https://www.sciencedirect.com
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Methods of Transfection
Source: https://www.google.com/search?q=DNA+uptake+by+cells&rlz
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Getting your gene into the cells Cells must be able to take up and incorporate the DNA into it’s genome Demonstrated by reporter genes (i.e. GFP) **Notice differences in intensity‐what does this mean????
Source: https://openlab.citytech.cuny.edu/
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Selection and Cloning Your cells are “polyclonal”‐meaning the cells have the gene, some have more copies of the gene You need to separate (i.e. select) these cells so that you have 1 cell type all containing the same number and location of the insert There are different methods to do this….
Source: https://www.euromabnet.com/protocols/cloning
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Screening Cell Line Candidates ICH Q5D‐urges biomanufacturers to begin each process with a clonal cell substrate Filter based on output Selection criteria
250
200
cell output
Looking for good output (PCD) Cell morphology (i.e. comparable to parental cell line)
Clonal output 300
150
Original Polyclonal Output
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50
0 90 98 57 24 75 17 79 37 59 44 35 34 20 33 30 28 51 67 66 50 10 83 7
6 41
clone designation
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Choosing a Clone Screening cell line candidates Good output (PCD) Stable output over many passages Normal doubling times (compared to parental) Consistent cell morphology
Clonal Output 300
250
200
150
100
50
0 60
9
63 Passage 1
6
Passage 4
Passage 8
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Passage 10
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Cell Banking Operations Objective: create and stably store cell banks for continual manufacturing and safety testing 44
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Cell Banks Seed Bank (usually 10‐20 vials) Master Cell Bank* (usually 100‐150 vials) 3‐tier system Working Cell Bank* (X00‐X000 vials) End of Production Cell Bank* (50‐100 vials) *store at multiple locations… WHY? 45
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Cell Bank Characterization Adventitious Agent testing
Viral (numerous tests‐in vitro, in vivo, PCR) Sterility (USP <71>) Mycoplasma (USP <63>, PtoC, PCR) Endotoxin (USP <85>)
Cell Stability (viability) and Genetic Stability (loss of insert/rearrangement‐restriction digests) Tumorigenicity (big for cell therapy applications) Comparison of output (from Master to End of Production) Morphology assessment (looking for consistency) Doubling times (looking for consistency) Points to Consider in the Characterization of Cell Lines Used to Produce Biologicals (1993) ICH guidelines (Derivation and Characterization of cell substrates used for the production of biotechnological/biological products)
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Why do all this development and characterization work? Cell Banks are critically important‐Company value Highly protected Limited access
Source: Cord Blood Banking Processscbb.com.sg
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Time for Regulatory Objective: successfully file a submission (i.e. and gain approval) with the FDA for the manufacturing of your investigational new drug (IND) for clinical use 48
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What is the FDA? What is the FDA? The FDA is a governmental body that provides guidance for bringing a drug, biologic or medical device to market
What does the FDA do? The FDA enforces rules governing the process for bringing a drug, biologic or medical device to market Combination product?
What authority does the FDA have? Where is the FDA?
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Ready for your IND Preclinical Testing Pharmacology and toxicology studies (is the drug safe for humans)
CMC (Drug Substance/Drug Product) Composition, manufacturer, stability, controls used for manufacturing the drug, consistency, aseptic validation, assays and qualifications
Investigator Information Qualifications for the investigator(s) who oversee the administration for the experimental drug
Clinical Trial Protocol Detailed protocol for the proposed clinical study and exposure to any risks (emphasized and scrutinized)
30‐day review period
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Clinical Trials and Beyond
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Clinical Trials Objective: successfully enroll a series of clinical trials that will be used to demonstrate the safety and efficacy of your new drug 52
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CMC Development
Refer to Current Good Manufacturing Practice for Phase 1 Investigational Drugs Guidance for Industry JULY 2008 53
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Ready for the clinic Phase I (usually small:10‐50 patients depending on the indication) Safety is the primary outcome Sometimes requested by the FDA to be staggered (especially for new technologies)
Phase II (larger population: 50‐X00’s patients) Continued safety and efficacy
Phase III (larger population: X00’s‐X000’s patients) Continued safety and efficacy
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Where are you going to Manufacture your B Antibody? Good question ‐This has to fit into previous 2 slides!!! Site Identification Facility Design‐Clean Spaces Facility Construction Validation Process Performance Qualification (PPQ) CFR part 211 Subpart C, Building and facilities [covers design and construction features, lighting, HVAC, plumbing, maintenance, etc.]
Source: https://pbn.com/
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More Regulatory Biologics License Application (BLA)
Applicant information Product/Manufacturing Information Pre‐Clinical Studies Clinical Studies Labeling
Form 356H
PAI (FDA inspection)‐”green light” Commercial Manufacturing
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Utilities Objective: become familiar with different utilities within a biopharmaceutical manufacturing plant 57
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Utilities HVAC Electrical Compressed Air Clean Compressed Air (CCA) Instrument Air
Water Purified water Water for Injection (WFI)
Steam Plant steam Clean steam
Compressed gases
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Utilities ‐ HVAC Heating, Ventilation, Air Conditioning Controls air borne particles, dust and microorganisms using high efficiency particulate air (HEPA) filters Maintain room pressure– Areas that must remain “cleaner” than surrounding areas must be kept under a “positive” pressurization, meaning that air flow must be from the “cleaner” area towards the adjoining space (through doors or other openings) to reduce the chance of airborne contamination. Provides adequate air changes/hour Maintain space moisture (relative humidity) Maintain space temperature
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Utilities ‐ Electrical Electrical Various supplies are needed 110 volt to 480 volt Single to triple phase
Emergency back up power To support critical equipment Typically has short duration delay
UPS To support critical equipment during delays
Source: https://cfeedu.cfemedia.com
Electrical supply is typically verified at points of use during validation
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Utilities ‐ Compressed Air Clean Compressed Air Systems Used to blow down systems Oil free compressor Requires Testing: Oils/hydrocarbons Vapor pressure dewpoint Particulates
Instrument Air Actuates valves in process lines/autoclaves
Source: https://www.airbestpractices.com
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Utilities ‐ Water Water for Injection (WFI) Used for final rinses during cleaning Product contact Subjected to testing:
Total organic carbon Bioburden Conductivity Endotoxin
Purified Water Used to feed stills and laboratory use Total organic carbon Bioburden Conductivity Source: http://kremesti.com/water
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Utilities ‐ Steam Clean Steam Used in cGMP autoclave for processing equipment and humidification Clean steam condensate meets WFI standards Generated from purified water using a clean steam still
Plant Steam Used for heating purposes (environmental conditions) Heat exchangers Potable water supply
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Utilities ‐ Compressed Gases Carbon Dioxide Nitrogen Liquid Nitrogen Subjected to testing Purity
Source: https://en.wikipedia.org
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Lock Out/Tag Out Safety concerns Do not operate Request information
Source: https://safetymanagementgroup.com/
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Gowning: Contamination Control Objective: successfully don gowning in a manner than substantially decreases the likelihood of contamination. 66
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Manufacturing Biopharmaceuticals in Cleanrooms A room in which the concentration of airborne particles is controlled and which is constructed and used in a manner to minimize the introduction, generation, and retention of particles inside the room and in which other relevant parameters, e.g. temperature, humidity, and pressure, are controlled as necessary.
Source: https://www.gotopac.com/art‐cr‐iso‐cleanroom‐classifications
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Gowning Do’s and Do Not’s Do gown‐in according to SOP Do not gown‐in if: You have an illness or medical condition that adversely affects the safety or quality of the drug product You have been exposed to the animal facility, wastewater treatment plant or laboratories that test for live viruses or mycoplasma (on the same day). You are wearing cosmetics of any kind or jewelry (excluding medical alert identification items)
No eating, drinking, smoking or wearing personal outer wear inside classified production areas and controlled unclassified spaces or utility areas
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Gowning Levels of gowning Level 1 Scrubs, lab coat, hairnet, booties, safety glasses (ISO 8)
Source: https://www.panelbuilt.com
Level 2 Scrubs, hairnet, booties, safety googles followed by hood, coverall, knee high boots, sterile gloves, goggles (ISO 7)
Level 3 Level 2 with sterile sleeves, a second layer of sterile gloves (ISO 5)
Gowning Qualification (testing and frequency) Source: https://www.aramarkuniform.com/
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Why gown? Requirement (both EU and FDA) Overall reduction of bioburden shedding Less microbial load in clean rooms Enhances microbial monitoring results Per Guidance for Industry. Sterile Drug Products Produced by Aseptic Processing‐ Current Good Manufacturing Practice A program that establishes, both initially and on a periodic basis, the capability of an individual to don the complete sterile in an aseptic manner. Plating operators (qualification)
Source: https://www.dphu.org
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Assessment
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Break
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Biomanufacturing Overview
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BioManufacturing Overview
Lyophilization
Source: https://www.researchgate.net/figure/The‐biopharmaceutical‐manufacturing‐technology‐flowchart
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Therapeutic Gene R&D and Product Development
Typical Biological Manufacturing Process Flow Diagram (Mab)
Expression Vector / Host Cell Line Development
ICH Q5A Q5B Q5D Q6E
Clone
Research Cell Bank (RCB) Cell Banking
Upstream Manufacturing
Q7
Master Cell Bank (MCB) Working Cell Bank (WCB)
USP Drug Substance Cell Culture Scale‐up N‐2, N‐1, N
Cell Culture / Seed Train / Bioreactor
Downstream Manufacturing
Harvest / Clarification
Q7
ICH Q5A Q5C Q5E Q6B Q11
• • • • • •
Purification Capture Viral Inactivation UF / DF Polish Viral Filtration UF / DF
Bulk Drug Substance Formulation & Fill
Clarified Bulk
ICH=International Conference on Harmonization Guidances USP=United States Pharmacopeia A typical biologic manufacturing process flow diagram with appropriate ICH guidance steps. (Source: Cytovance Biologics Inc. John Conner, 2013.)
DSP Process Drug Product
Drug Product Formulation & Sterile Formulation & Fill
Q5E, Q6B, Q8
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First and Foremost: cGMP/Good Documentation Practices GDP is included in cGMP
Standard operating procedures (SOP) Specifications Validation documents Batch records Product and sample/Status labels
The FDA can inspect the facility at any time….Surprise!!!!!
Good Documentation Practice ...presentationeze.com
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Media Prep A water‐based nutrient solution that contains defined amounts of salts, buffers, sugars and proteins in which the cells live. Nutrient media is added to all single use systems and stainless‐steel bioreactors Objective: Manufacture media for cell growth (inoculum through final bioreactor) 77
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Media Types of Media: MEM
MEM is a modification of Basal Medium Eagle (BME) which contains a higher concentration of amino acids and vitamins, as well as additional supplementary components
DMEM–Dulbecco's Modified Eagle Medium Hams F12
Source: https://www.fishersci.com
Supplements
Glutamax in place of glutamine Protein source (plant Vs animal)
Cell and Gene Therapy vs. Large scale
Bottles vs. prepared on site from powders Both scenarios involve a hold period For large volumes, media trains utilize filtrations as a means to sterilize the media (housings constructed of 316Lss) Source: https://www.jobvector.ch
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Did you know???.... The raw materials used to prepare media are assessed for quality and sterility prior to being sent to upstream laboratories for media preparation and use.
Supplier and Raw Materials ...bioprocessintl.com
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Media Prep: Process Parameters Hold storage conditions WFI temperature pH Osmolality Why are these important????
Microbial Control
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Media Prep: Performance Indicators pH Pre‐filtration osmolality Pre‐filtration bioburden Why are these important????
Microbial Control
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Courtesy of Amgen, Inc
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Inoculum Objective: successfully initiate a culture‐ this is likely an “open system” and requires training. 83
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Cell Thaw: Inoculum WCB vial is removed from cryostorage unit (‐196˚C) Rapidly thawed (important‐why?) Removal/dilution of cryoprotectant Resuspended Cell count and viability assessment (automated systems available for determining viability and cell number) Viability is historically measured using trypan blue exclusion methodology
Source: www.gmi‐inc.com Source: www.planar.com
Source: www.fishersci.com
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Cell Thaw: Inoculum Open system (risk) Work is done in a Biological Safety Cabinet (ISO 5) or isolator High air changes/hour HEPA filtered air Protects operator and the product Use of flasks or other culture vessel (i.e. bottle, spinner)
Source: www.triumvirate.com
The LFH protects only the product in the hood such as sterile media, while the BSC protects the user and the product in the cabinet from bacterial contamination. Note direction of airflow
Source: www.fishersci.com Source: www.fishersci.com Source: www.fishersci.com
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Inoculum: Process Parameters Temperature Gas Agitation Culture duration Why are these important????
Microbial Control
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Inoculum: Performance Indicators Final viable cell density Final viability Why are these important????
Microbial Control
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Lab Aseptic Processing Cell Viability
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Aseptic Processing‐ Cell Thaw Equipment and Raw Materials Gowning Trained Staff Cell Thaw Personnel Monitoring Environmental Monitoring of BSC/LFU
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Equipment and Raw Materials Examples: Equipment ID BSC ‐001 BSC‐002
Certification Date 12/30/2020 12/31/2020
Certification Due Date 12/30/2021 12/31/2021
Minihelic Reading 0.25” 0.25”
Initial/Date CM 10/3/2021
Media Type Touch Plates
Manufacturer Remel
Media Lot Number 9280464
Date of Expiration 12/05/2021
Initial/Date CM 10/3/2021
Cell Culture Media IMX
Manufacturer
Media Lot Number
Date of Expiration
Initial/Date
Amgen
9280464
12/05/2021
CM 10/3/2021
What do you think it takes to use these?
100% Team Sport
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Typical Gowning Scenarios ISO 7 ISO 5
ISO 8
https://www.lifescienceleader.com
https://industry24h.com https://www.criticalenvironmentsolutions.co.uk
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Why go to the trouble of gowning? Requirement (both EU and FDA) Overall reduction of bioburden and particulate shedding Less microbial load in clean rooms Enhances microbial monitoring results Gowning training and qualifications are always a favorite request of FDA inspectors and QPs (EU). Important to have up to date training records
Amgen Training Workshop September, 2019
Baseline Reading SAS sample (200L)
Forced Failure (3‐5 second beard scratch) SAS sample (200L)
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Aseptic Cell Thaw (video)
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Cell Viability/Cell Count Differentiate between live and dead cells Trypan Blue mechanism of action Manual vs. Automated
Source: www.fishersci.com Source: www. https://custombiotech.roche.com
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Determining Cell Number Count cells as follows: Clean, thoroughly dry, and assemble the hemocytometer with the cover slip. Transfer a small amount of cell suspension to the edge of each of the two counting chambers. Allow the cell suspension to be drawn into the counting chamber by capillary action. Place the hemocytometer under an inverted microscope and view the cells under magnification. Focus on the quadrants, labeled 1, 2, 3, and 4. Record the number of cells in each section. Average the number of cells, and multiply by the dilution factor. If the cells have not been diluted, this factor will be 10⁴ cells/mL. Any dilution of the sample after it was removed from the cell suspension, such as using vital stain, needs to be included in the calculation.
Source: https://www.hemocytometer.org/
95
95
Determining Viable Cell Number Quick Calculation 𝑁𝑢𝑚𝑏𝑒𝑟 𝑜𝑓 𝑉𝑖𝑎𝑏𝑙𝑒 𝐶𝑒𝑙𝑙𝑠 𝑁𝑢𝑚𝑏𝑒𝑟 𝑜𝑓 𝑉𝑖𝑎𝑏𝑙𝑒 𝐶𝑒𝑙𝑙𝑠 𝑁𝑢𝑚𝑏𝑒𝑟 𝑜𝑓 𝑁𝑜𝑛𝑣𝑖𝑎𝑏𝑙𝑒 𝐶𝑒𝑙𝑙𝑠
From the hemocytometer:
𝑋 100
live
Number of Viable Cells: 69 Number of Nonviable Cells: 13 Dead
69 69
13
𝑋 100
Viability = 84%
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Cell Viability (video)
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Image (Cell Viability)
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Calculation (Cell Viability) Quick Calculation From the hemocytometer count XX live cells and XX dead cells Determine Viability x 100%
The cell preparation is XX % viable
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Calculation (Cell Viability) Quick Calculation From the hemocytometer we counted 20 live cells and 2 dead cells Determine Viability x 100%
x 100%= 91%
The cell preparation is 91% viable
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Calculation (Cell Count) Given Information Sample removed from a 20 ml cell suspension A 1:10 dilution of the sample was prepared and counted (50µL cell suspension into 450µL trypan blue)
Determine cells/mL and total cells x 104 x dilution factor
#
x 104 x 10 = 5.0 x 105
Now multiply by the total cell suspension volume (i.e., 20 mL) to get total cell number: 5.0 x 105
x 20 mL= 10 x 106 cells 101
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Lunch
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Cell Scale Up Objective: successfully increase your cell numbers of sequential cell culture operations to seed a final production reactor. 103
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Cell Scale Up
Source: www.eppendorf.com
Source: www.americaninstrument.com
After defined time, cells are processed (may mean trypsinization for adherent cell lines), and enumerated to get a total cell count. Typically a multistep process Following this, cells are used to seed the production reactor(s). Both transfers from inoculum through scale‐up are typically (not always) closed systems (emphasis on closed systems).
Source: www.murraycompany.com
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Scale Up: Process Parameters Target seed density Temperature Gas Agitation Culture duration Why are these important????
Microbial Control 105
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Scale Up: Performance Indicators Final viable cell density Final viability Why are these testing important????
Microbial Control 106
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Bioreactors Key Features: Materials of Construction Probes Temperature pH (indicative of cellular waste) Dissolved oxygen (DO)
Agitation Antifoam addition Sampling ports SIP system‐closed Nutrients (glucose, protein, etc.)
Source: https://pediaa.com/difference‐between‐bioreactor‐and‐fermentor
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The process would look like this…… SUS (wave or SUB) Can simplify the process Efficient Shorter runway Utilizes prevalidated (cleaning) materials
BioProcess International, March, 2015
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Single Use Systems (SUS) Batch to the Future: Stainless Steel Continues to Shine (Bioprocess International West, March, 2019) Samsung BioLogics Celltrion Fujifilm Diosynth Biotechnologies
Recently build facilities using stainless steel
Cited concerns include:
Particulates (BioProcess International, April, 2019) Leachable (compromise cell viability and growth) “Close it up”….impact on COGs Leaks (manual connections)
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Single Use Systems (SUS) Still a strong movement towards SUS (paradigm shift)
WuXi AGC Bio Patheon Catalent
Recently built facility using SUS
Can a 1000L SUS equal to 10,000L 316L ss bioreactor (g/L to 10g/L) Yes, the smaller facility footprint will work Historically, add bioreactor suites to increase output More recently, optimization of production media (multiple grams/L) Enhancers added to media
Now, attention has shifted from media to the cell line (10 g/L) Characteristics which increase cell viability and improve expression titers
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Impact on Facility……. Construction time….15 months Cost….quarter of the capital cost Highly sustainable environmental footprint 80% less energy and water 75% reduction in carbon dioxide emission levels
75% smaller than a conventional facility Still able to deliver the same quantity and quality of products
Source: www.amgen.com
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Regardless of 316Lss or SUS….. Process parameters: Temperature (maintain 36°C) pH (maintain around pH 7.0) Nutrients (maintain [glucose], [protein], etc.) Dissolved oxygen Antifoam Target seed density Culture duration
Microbial Control
Source: https://pediaa.com/difference‐between‐bioreactor‐and‐fermentor
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Regardless of 316Lss or SUS….. Performance indicators: Final viable cell density Final viability
Microbial Control
Source: https://pediaa.com/difference‐between‐bioreactor‐and‐fermentor
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Types of Manufacturing Processes
Source: https://www.semanticscholar.org
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Characteristics of Batch, Fed Batch and Perfusion Systems Batch Add materials at the start, production is lower (1X) Dominated the industry Originally used for smaller quantities
Fed Batch Media addition to culture increasing yield up to 2X‐3X Increase production with modest increases in COGs
Perfusion Perfusion cell culture to increase production up to 10X Cost effective
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Lab Bioreactors
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Introduction to Bioreactors Cells (adherent vs. suspension) T‐flasks, Roller Bottles, Cell Factories/Cubes, Culture Bags, and Shaker Flasks
Expression of POI (protein of interest) Freestyle Cell Line and media 117
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Bioreactors Key Features: Materials of Construction Probes Temperature pH Dissolved oxygen (DO) Agitation Antifoam addition Sampling ports SIP system‐closed Nutrients (glucose, protein, etc.)
Source: https://www.labcompare.com
Source: https://www. www.b2bcentral.co.za
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Cell Bioreactors (Video)
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Recent BioFlo Run (1001 Data) BioFlo Run 1001‐ Temperature 38
Temperature (deg C)
37.8 37.6 37.4 37.2 37 36.8 36.6 36.4 36.2 36 94 91 88 85 82 79 76 73 70 67 64 61 58 55 52 49 46 43 40 37 34 31 28 25 22 19 16 13 10 7 4 1 Time (hours)
Process Value Setpoint
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Recent BioFlo Run (1001 Data) BioFlo Run 1001‐ pH 8 7.8 7.6 7.4
pH
7.2 7 6.8 6.6 6.4 6.2 6 94 91 88 85 82 79 76 73 70 67 64 61 58 55 52 49 46 43 40 37 34 31 28 25 22 19 16 13 10 7 4 1 Time (hours)
Process Value
Setpoint
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Recent BioFlo Run (1001 Data) BioFlo Run 1001 Dissolved Oxygen 38
37
Dissolved O2 (%)
36
35
34
33
32 94 91 88 85 82 79 76 73 70 67 64 61 58 55 52 49 46 43 40 37 34 31 28 25 22 19 16 13 10 7 4 1 Time (hours)
Process Value Setpoint
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Lab Mixing
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Mixing Importance of Mixing Media/Cell Suspension/Buffers/Product Pools Vessel Shape Impellor Type Speed Cell Shear Foam Generation Vortex
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Impellers:
Gentle Marine Blade Impellers Pitched Blade Impellers
Source: BioProcess International; January, 2009
Rushton Impellers
What do you think the difference is? 125
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Mixing Study (Video)
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Break
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Cell Harvest Objective: successfully separate your workhorse cell line from the production media. 128
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Cell Harvest
Courtesy of Amgen, Inc.
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Courtesy of Amgen, Inc.
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Cell Harvest Cell separation is achieved by filtration or centrifugation.
Celeros APD‐250 Centrifuge
challenges
Different commercially available methods In the end, the media is what we want Contained in a harvest tank May require additional processing before concentration
Source: www.celeros‐separation.com
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Product Concentration The membrane retains the larger macromolecules while allowing the flow of smaller molecules, media, and media components. Substantially decreases the overall volume of the suspension decreasing the volume that will go over the column in subsequent steps.
Depth Filtration System Source: BioProcess International, May, 2012
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Process Parameters Filtration Filter area Flow rate Differential pressure during filtration
Why are these important????
Microbial Control
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Neutralization: Performance Indicators Neutralization pH Acidic peaks Bioburden
Why are these important????
Microbial Control
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Filtration: Performance Indicators Post‐harvest bioburden Why is this important????
Microbial Control
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Downstream Purification
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Therapeutic Gene R&D and Product Development
Typical Biological Manufacturing Process Flow Diagram (Mab)
Expression Vector / Host Cell Line Development
ICH Q5A Q5B Q5D Q6E
Clone
Research Cell Bank (RCB) Cell Banking
Upstream Manufacturing
Q7
Master Cell Bank (MCB) Working Cell Bank (WCB)
USP Drug Substance Cell Culture Scale‐up N‐2, N‐1, N
Cell Culture / Seed Train / Bioreactor
Downstream Manufacturing
Harvest / Clarification
Q7
ICH Q5A Q5C Q5E Q6B Q11
• • • • • •
Purification Capture Viral Inactivation UF / DF Polish Viral Filtration UF / DF
Bulk Drug Substance Formulation & Fill
Clarified Bulk
ICH=International Conference on Harmonization Guidances USP=United States Pharmacopeia A typical biologic manufacturing process flow diagram with appropriate ICH guidance steps. (Source: Cytovance Biologics Inc. John Conner, 2013.)
DSP Process Drug Product
Drug Product Formulation & Sterile Formulation & Fill
Q5E, Q6B, Q8
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Buffer Prep Solutions in which the pH remains relatively constant even when small amounts of acid or base are added: Objective: Manufacture buffers for purification operations 138
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Did you know??? The raw materials used to prepare buffers are assessed for quality and microbial control prior to being sent downstream for buffer preparation and use.
Amgen, Inc. 139
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Why Use Buffers? Buffers are used to protect the protein from changes in pH by buffering or absorbing changes in pH. A well‐buffered solution will maintain its pH in spite of variations in processing, containers, and raw materials. Proteins are sensitive to changes in pH, which can lead to denaturation, aggregation, and fragmentation. Types of buffers Phosphate, citrate, acetate and tris‐based buffers (as examples) Each have different buffering (pH controlling) capacities and are used at different steps in the biomanufacturing process.
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Buffers Below is a partial list of buffers used at Amgen, Inc. Growth promoting buffers are those that may be more susceptible to bacterial growth!!
Courtesy of Amgen, Inc.
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Buffer: Process Parameters Buffer Preparation Temperature pH and/or conductivity Agitation
What are you testing for, and when to ensure control? Bioburden, endotoxin, conductivity, and pH Close to use
Microbial Control
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Protein Purification Objective: successfully separate your protein from all the other components in the production media. 143
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Courtesy of Amgen, Inc.
Please note that the order of the chromatographic processes may change depending upon the protein that is being purified. Typically, purification begins with Protein A chromatography 144
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Protein Purification What is Column Chromatography? Column chromatography is a common technique used to separate individual compounds from a mixture.
A volume is layered over the column, washed, and collected (i.e. eluted)
Source: https://www.thermofisher.com
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Types of Chromatography Type of Chromatography Affinity
MOA
Binds with:
A specific interaction Non competing ligand
Ion Exchange
Net surface charge
Low ionic strength
Hydrophobic Interaction
Hydrophobicity
High ionic strength
Size Exclusion
Hydrodynamic radii
Separation based on hydrodynamic size
Elute with:
Competing ligand (specific); conditions that disrupt protein/protein interactions (non‐ specific) High ionic strength; Increased (cation exchange) or decreased (anion exchange) pH Low ionic strength
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The Stationary Phase Stationary Phase: Chromatography occurs with a solid support (often called a resin or matrix) packed into a column forming the stationary phase. Protein A (can be native or recombinant) Similar Fc regions to IgG but recombinant has been engineered to include a C‐ terminal cysteine that enables a single point coupling to Sepharose increasing binding capacity.
Source: https://en.wikipedia.org
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The Mobile Phase Mobile Phase: The mobile phase, a solution containing a mixture of molecules, is moved through the column from one end to the other. The chemical and physical differences in the molecules leads to different rates of passage through the column matrix, leading to separation.
Source: https://en.wikipedia.org
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Wash Buffers Wash Buffer Characteristics: Once the binding interaction occurs, the support is washed with additional buffer to remove non‐bound components of the sample. [Nonspecific (e.g., simple ionic) binding interactions can be minimized by moderate adjustments to salt concentration in the binding and/or wash buffer]. Can also be a change in pH.
Typical wash buffers: Phosphate buffers Tris buffers Source: https://en.wikipedia.org
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Elution Elution Buffer Characteristics: Break the binding interaction of the target molecule and releases it Dissociate binding by changes in: pH (low or high) high salt (ionic strength)
Subsequent dialysis or desalting is required to exchange the purified protein from elution buffer into a more suitable buffer for storage or downstream analysis. Typical Elution Buffer: 100mM Sodium Acetate, pH 3.7
Source: https://en.wikipedia.org
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Monitoring Methods for Monitoring:
SDS page of fractions FTIR HPLC UV Detection
Monitoring the presence (or absence) of peaks is key to determining if the therapeutic protein has been separated properly! Know what to look for!! Source: https://www.researchgate.net
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Protein Purification: Chromatography Process parameters (examples)
Load Factor Flow Rates Volumes Number of Cycles
Performance indicators (examples)
Bioburden Endotoxin SE‐HPLC Impurities (Host Cell Protein, DNA) Leached Protein A
Microbial Control
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Assessment
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Day 1 Wrap Up and Evaluation
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Day 2
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Biochemistry 101 & Downstream Purification 156
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Background Biochemistry 101 What is a Protein? What are its structural components? Linkage between protein amino acid sequence and 3D shape? Size‐Charge‐Hydrophobicity distribution in complex samples? Changes in protein structure – denaturation? Protein Aggregation?
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Four levels of protein structure
Amino Acid Sequence
B‐Sheet α‐Helix
3D folded Tertiary structure
Multi‐subunit Quaternary 3D Structure
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Know your protein!
Human Serum Albumin
Primary Amino Acid Sequence MKWVTFISLL LLFSSAYSRG VFRRDTHKSE IAHRFKDLGE EHFKGLVLIA FSQYLQQCPFDEHVKLVNEL TEFAKTCVAD ESHAGCEKSL HTLFGDELCK VASLRETYGMADCCEKQEP ERNECFLSHK DDSPDLPKLK PDPNTLCDEFKADEKKFWGK YLYEIARRHP YFYAPELLYYANKYNGVFQE CCQAEDKGAC LLPKIETMRE KVLTSSARQR LRCASIQKFG ERALKAWSVA RLSQKFPKAE FVEVTKLVTD LTKVHKECCH GDLLECADDR ADLAKYICDN QDTISSKLKECCDKPLLEKS HCIAEVEKDA IPENLPPLTA DFAEDKDVCK NYQEAKDAFL GSFLYEYSRR HPEYAVSVLL RLAKEYEATL EECCAKDDPH ACYSTVFDKL KHLVDEPQNL IKQNCDQFEKLGEYGFQNAL IVRYTRKVPQ VSTPTLVEVS RSLGKVGTRC CTKPESERMP CTEDYLSLIL NRLCVLHEKT PVSEKVTKCC TESLVNRRPC FSALTPDETY VPKAFDEKLF TFHADICTLPDTEKQIKKQT ALVELLKHKP KATEEQLKTV MENFVAFVDK CCAADDKEACFAVEGPKLV WSTQTALA
MWt. (molecular weight) = 69,000 Daltons (69 kD) pI (isoelectric point) = 5.82 Hydrophobicity index = ‐ 0.395 159
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Protein chemistry ‐ MWt. distribution
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Protein Chemistry – Charge distribution
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Protein Chemistry – Hydrophobicity
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Loss of native structure (denaturation)
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Protein Aggregation
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Downstream Processing
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How do you purify a product?
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What protein properties can you exploit in developing a separation?
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Factors influencing Size/Shape based separations – Stokes Radius effects Impact on charge state can lead to unfolding and change in shape Neutralize ionic interactions leading to a change in shape Promote Protein‐Protein interactions leading to aggregation Can promote aggregation Change protein diffusion rate and can impact kinetics Loss of disulfide bonds can lead to unfolding Can aid in solubility (membrane proteins) but also lead to denaturation Promote unfolding and denaturation
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Factors influencing a charge‐based separation
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Factors influencing hydrophobic interaction (HIC) based separation Direct influence on the overall hydrophobicity of the target protein – membrane proteins Neutralize ionic interactions at high ionic strength Can impact protein solubility and HIC separation Increase in temperature promotes HIC interactions Can lead to changes in the hydration state of a protein due to un‐ folding of protein structure, Can impact kinetics of protein interaction with the stationary phase and local diffusion limitations. HIC surfaces can offer a range of hydrophobicity leading to varying degrees of retention/elution. 170
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Assessment
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Break
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Chromatography I Modes
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Chromatography Modes Size exclusion/gel permeation (SEC) Ion exchange (IEX) Hydrophobic interaction (HIC) Biospecific Recognition – Affinity Chromatography Mixed mode
174 174
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Size exclusion/gel permeation
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Variables influencing IEX Chromatography • Choice of IEX chemistry, • pI range of sample, • pH of equilibration buffer, • Ionic strength, • Presence on non‐ionic components (glycerol, urea, detergents etc), • Residence time in contact with IEX media (flow rate, column geometry). 176
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Ion exchange (IEX) mode
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Example ‐ IEX fractionation of plasma Basic pH optimization with NO salt elution
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Hydrophobic interaction (HIC) HIC ligands
Hoffmeister Series of Counter ions
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Example of a HIC separation
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Mixed Mode Separation
181
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Example of Mixed Mode ‐ Flow through polishing of a mAb after Protein A capture
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Bio‐specific Recognition (Affinity)
183
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Components of an Affinity Resin
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Affinity Chromatography Workflow
185
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Affinity Activation Chemistries
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Affinity Ligands
187
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Protein Purification Applications Monoclonal Antibody (mAb) capture; rProtein A affinity‐based purification of antibodies
from cell culture medium, Direct capture on cation exchange resin.
Polishing of captured mAb to remove impurities;
IEX chromatography, HIC, Hydroxyapatite, Mixed mode (AEX/HIC)
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rProtein A Affinity Capture
189
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Recent improvements to rProtein A
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Direct Capture by Cation IEX
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Capture‐polishing process integration ‐ Protein A capture followed by IEX and mixed mode polishing
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Please note that the order of the chromatographic processes may change depending upon the protein that is being purified. Typically, purification begins with Protein A chromatography
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Overview of AMGEN multistep purification process for a mAb – Capture from cell culture
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Overview of AMGEN multistep purification process for a mAb ‐ Polishing Polishing Step 1 – low pH viral inactivation, Polishing Step 2 – Mixed mode AEX (Capto Adhere MMC);
157 L column volume, mAb Flow Through mode, High mAb recovery (> 80%), Slight increase in volume, Removes CHO‐HCP, dsDNA, leached Protein A, mAb aggregates, viruses and endotoxin
Polishing Step 3 – Cation Exchange (Fractogel‐S CEX) chromatography; 308L column volume, Bind and elute mode, Removes mAb dimers, aggregates and CHO‐HCP.
Polishing Step 4 – Viral filtration. UF/DF to condition the final mAb product for formulation 195
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Assessment
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Lunch
197
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Chromatography II Applications
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Trends in Bioprocess
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Bead types improvements in mass transport
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Membrane Absorbers improvements in mass transport and flow rate balanced with lower capacity
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Hybrid Membrane Absorbers improvements in mass transport, flow rate and capacity
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Cross‐linked Agarose
203
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Fibrous Membrane Absorbers improvements in mass transport, flow rate and but still lower capacity?
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Properties of Large‐Scale Bioprocess Chromatography Media
205
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Continuous Bioprocessing
206
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Multicolumn Bioprocessing
207
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Summary
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Assessment
209
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Break
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Lab Protein Purification
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Day 2 Wrap Up and Evaluation
212
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Day 3
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Viral Interaction/Removal Objective: successfully remove or inactivate any potential viruses in your protein. 214
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What are we removing?
Mammalian cells Used for protein production
Contamination Source: https://gut.bmj.com
Contamination
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Viral Anatomy Capsid (outer protein coat) Genome RNA viruses DNA viruses
Shape Variation Helical, icosahedral, polyhedral, spherical
Size variation
Parvovirsuses‐20‐25 nm Circovirus‐18‐25 nm Retroviruses‐80‐100 nm Mimiviridae‐ 500 nm
Source: www.anipedia.com
Source: www.arstechnica.com
Source: www.sciencephoto.com
Source: www.sciencephoto.com
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Covid‐19 Enveloped 20 nm club shaped glycoprotein projections
Genome RNA viruses (positive sense, ssRNA) Approximately 26‐32 Kbp
Appearance Halo/crown like
Shape Variation Spherical/pleomorphic form
Size variation 80‐120 nm (variable references)
Source: S. Sikotra, Leicester Royal Infirmary, England
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Viral Reduction When does it occur? At the very beginning… Sourcing raw materials Examples? 9CFR
Qualifying vendors who can provide the appropriate documentation. Appropriate validated manufacturing and test methodologies Substituting plant proteins
Source: www.bestlifeonline.com
During Manufacturing Low pH buffers Temperature exposure Solvent/detergent
During facility/equipment cleaning Source: www.agric.wa.gov.au
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Viral Inactivation and Removal Specific steps for viral inactivation Heat (Primatone) Acid (low pH)
Very effective
Nanofiltration (similar to FBS production process) Inactivation can be incorporated into multiple positions of the manufacturing process Typically towards the end of the process
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Viral Removal (Filtration)
Source: BipPharm International Volume 19, Issue 10
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Viral Removal (Filtration)
Source: Planova filters: virus removal for biotherapeutic products
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221
Viral Removal (Filtration)
Source: Planova filters: virus removal for biotherapeutic products
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Viral Removal (Filter Integrity)
The Ashai Gold Particle Test System: • Automated • Validated • Minimizes operator error • Provides assurance of post use filet integrity
Source: Planova filters: virus removal for biotherapeutic products
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Viral Validation Studies
Source: BipPharm International Volume 19, Issue 10
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UF/DF Objective: Successfully concentrate the therapeutic to its final formulation and exchange the buffer to one that is preferred for storage stability and ease of administration. 225
225
What is Ultrafiltration/Diafiltration(UF/DF)? • The UF step is a concentration that reduces the amount of volume of the product by separating the molecules based on the membrane pore size or molecular weight cutoff. • The DF is a diafiltration step that exchanges one buffer solution with another (final formulation buffer). UF/DF can include Tangential Flow Filtration (TFF).
https://www.google.com/url?sa=i&url=htt ps%3A%2F%2Fwww.bpesys.com%2FPDF% 2Fultrafiltration‐diafiltration‐tff‐fact‐ sheet.pdf&psig=AOvVaw2g9oVguDAXGrs8 eqfihn7A&ust=1616676132094000&sourc e=images&cd=vfe&ved=2ahUKEwiUxOqF‐ sjvAhXDDt8KHZM‐D3EQr4kDegUIARCFAg
https://www.emdmillipore.com/Web‐US‐Site/en_CA/‐/USD/ShowDocument‐Pronet?id=201306.5278
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What Tangential flow filtration (TFF)? TFF is a cross‐flow filtration process used for separation of protein and particles. The fluid passes parallel to the membrane filters, rather than being pushed through a membrane perpendicularly. Particles that pass through the membranes flows to what is called the permeate side then to drain. The rest of the molecules (protein) flow across the membranes and are recycled back into a feed tank. https://www.logcheck.com/wp‐ content/uploads/2018/05/Slide1.jpg
Retain the Retentate! 227
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Ultrafiltration/Diafiltration (UF/DF) Process parameters (examples) Load Factor Flow Rates TMP Number of Cycles Diafiltration Buffer (pH, Osmolality) Performance indicators (examples) Bioburden Endotoxin pH Osmolality SE‐HPLC
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Drug Substance Release Testing Objective: successfully test your product for important attributes during the manufacturing process to ensure quality. 229
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Drug Substance Testing Appearance: Color, Clarity Identity: ELISA Purity: cIEF, SE‐HPLC, rCE‐SDS, Adventitious Agents: Bacterial Endotoxins, Bioburden Potency: Bioassay Quantity: protein concentration pH Osmolality Polysorbate 20
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Vial Filling Objective: successfully package your protein for storage and distribution. This function is performed outside of RI (Puerto Rico) 231
231
Vial Filling Aseptic Process (always validated) Automated process (isolator and/or strict ISO classifications)
Source: www.ivtnetwork.com
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Vial Filling Steps and Equipment Vial Wash and Depyrogenation Filling, Stoppering, Lyophilization, Crimping, Visual Inspection
Source: https://www.youtube.com/watch?app=desktop&v=tnaefPcN3mE
Source: https://www.emergentbiosolutions.com
Source: https://www.contractpharma.com
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Drug Product Release Testing Objective: successfully test your final product for important attributes prior to release to ensure quality. 234
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Drug Product Testing Appearance: Color, Clarity Identity: ELISA Purity: SE‐HPLC, CE‐SDS, RP‐HPLC, SDS‐PAGE Adventitious Agents: Bacterial Endotoxins, Sterility Potency: Bioassay Quantity: Protein Concentration pH Osmolality Polysorbate 20 Particulates
235
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Break
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Equipment Cleaning
237
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What are we removing?
Mammalian cells Used for protein production
Contamination Source: https://gut.bmj.com
Contamination
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Contamination Control Aseptic technique is critically important during the entire biomanufacturing process. Cleaning and sterilization of equipment must be performed on a regular basis Potential contamination sources of product include bacterial, fungal and viral from many different sources. Source: www.americanpharmaceuticalreview.com
Contamination at any stage of the biomanufacturing process is extremely expensive to mitigate; especially viral contamination!! 239
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Types of Equipment Cleaning Clean‐in‐Place (CIP)‐without assembly (automated chemical cleaning system) Large pieces of equipment…
Bioreactors Media and Buffer tanks Strong Acid and Base WFI rinses and monitored by pH
Clean out of Place (COP) Small pieces of equipment
Similar Challenges Complete coverage Complete removal of raw materials and cleaning agents Validation
Fixtures, clamps, fittings, etc. Washer system (Lancer)
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CIP Process Pre‐rinse with WFI (water for injection) or PW (purified water)
wets the interior surface of the tank and remove residue provides a non‐chemical pressure test of the CIP flow path.
Caustic solution single pass flush through the vessel to drain. Caustic is the main cleaning solution Caustic solution re‐circulation through the vessel Intermediate WFI or PW rinse Acid solution wash – used to remove mineral precipitates and protein residues. Final rinse with WFI or PW – rinses to flush out residual cleaning agents Final air blow – used to remove moisture remaining after CIP cycle Source: www.pharmtech.com
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Cleaning Validation is a must…… Smaller items cleaned in a glass washer can be challenged using organic carbon (i.e. sucrose) and rinses can be submitted for TOC analysis. Vessels can be challenged with riboflavin and visually inspected Riboflavin fluorescence under UV light and can easily be detected. Source: Sani‐Matic, Inc.
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Sterilization
Objective: Absence of viable organisms
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Sterilization Steam in Place (SIP)‐without assembly Large pieces of equipment… Bioreactors, media and buffer tanks, process piping Maintain a temperature of 121.1˚C for desired time Requires validated
Autoclaves Smaller pieces of equipment
Fixtures, clamps, fittings, etc. Generally double wrapped Established load patterns Established sterility shelf life (TBD) Maintain a temperature of 121.1˚C for desired time Requires validated
Similar Challenges Complete sterilization Validation
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Autoclave: Sterilization out of place Purge Phase
Steam flows through the sterilizer beginning the process of displacing the air; temperature and pressure ramp slightly to a continuous flow purge.
Exposure (Sterilization) Phase
During this phase, the exhaust valve closes causing the interior temperature and pressure to ramp up to the setpoint. The program then maintains the desired temperature (dwells) until the desired time is reached.
Exhaust Phase
The pressure is released from the chamber through an exhaust valve and the interior is restored to ambient pressure, although contents remain relatively hot.
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GMP Autoclave Clean steam supply (sampling port) Instrument air 316L ss construction Controller Thermocouple located in drain (cold spot) Dirty and clean sides (single vs. double door configurations)
Source: www.aoghmedical.com
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Steaming Validation is a must…… For autoclaves, a load pattern is established and validated using thermocouples and biological indicators. For bioreactors, media and buffer tanks, and process piping a similar approach is used. Typically B. Stearothermpohilus is used as an indicator. Growth at 55°C‐ 60°C is monitored. Must be negative for growth. TC/BIs are snaked into autoclave pouches and process piping TC/BI are distributed in autoclave chamber and vessels Must maintain 121.1 °C for exposure period Typically 3 consecutive runs are performed (both for load patterns and reactors)
Source: https://iopscience.iop.org
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Aseptic Processing Runs…… Once load pattern and/or process parameters are established, equipment is sterilized and then tested using TSB (tryptic soy broth) Typically performed as 3 consecutive runs Samples are collected for sterility testing Added assurance
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Alternative Sterilization Methods Objective: Absence of viable organisms
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Irradiation Methods Gamma Used in the syringe manufacturing process (also, needles, tubing, bags) Validated with sublethal dose Dose audits conducted quarterly
E‐beam (Electron beam) Used in medical device manufacturing (attention to adhesives and polymers) Validated with sublethal dose Dose audits conducted quarterly
UV (ultraviolet) Used for surface treatments (BSC)/isolators
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Facility Cleaning Objective: successfully minimize adventitious agent contamination through the use of appropriate disinfectants. 251
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Facility Cleaning Levels of cleaning Disinfection‐destroys microbes from surfaces (typical disinfection agents include Lysol (phenolic), quaternary agents (ammonium compounds), bleach, peroxide) Almost always effective against spore forming bacteria (but not always sporicidal‐example Sporicidin)
Sanitization‐reduces the number of microbes. Typically performed with IPA (70%). Not very effective against spores Some viricidal properties
Sterilization‐process of full destruction of microbes including those that are spore forming
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Facility Cleaning‐Cleaning Agents Vesphene, LpH, Vestasyde
Kills broad range of microorganisms Typically applied daily Contact time with little residue following rinsing Quick destruction of microorganisms Historically rotated on monthly basis (philosophy is changing)
Frequency Critical areas Flooring and horizontal surfaces are cleaned daily Walls and ceilings are cleaned monthly Sporklenz cleaning is preformed quarterly (ceilings, walls, and floors)
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Assessment
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Break
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EM‐Microbiology Objective: become familiar with different microbes and the importance of gram status. 256
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What are we looking for?
Mammalian cells Used for protein production
Contamination Source: https://gut.bmj.com
Contamination
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Different Bacterial Shapes EM is your report card Bacteria come in various shapes:
Cocci or round/spherical Bacillus or rod‐shaped Spiral or twisted Variable
Source: www.imagesofbacteria.blogspot.com
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The Gram Stain Developed by the bacteriologist Hans Christian Gram in 1884 Gram staining differentiates bacteria by the chemical and physical properties of their cell walls by detecting the presence of the peptidoglycan, which is present in the cell wall of Gram‐positive bacteria. Consists of 4 steps: Application of
Reagent
Primary Dye Trapping Agent Decolorizer Counterstain
Crystal violet Iodine Alcohol Safarin/carbol fuschin
Color Gram Positive Gram Negative purple purple purple purple purple colorless purple pink
Be careful with this step
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Bacterial Wall Structure
Why is gram status so important?
Source: https://www.researchgate.net
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The Gram Stain
Source: https://www.onlinebiologynotes.com
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Common Bacteria
E. coli
B. subtillus
S. aureus
Source: https://www.researchgate.net
Source: https://www.gettyimages.com
Source: https://en.wikipedia.org
S. epidermis Source: https://http://faculty.weber.edu
P. aeruginosa Source: https://en.wikipedia.org
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Endotoxin Gram negative microbes shed endotoxin Endotoxins are large molecules consisting of a lipid and a polysaccharide composed of O‐antigen, outer core and inner core found in the outer membrane of Gram negative bacteria. Effects include: Inflammation (TASS) Altered gene transcription
Detectable Gel clot method Chromogenic method Turbidimetric method Source: www.abbkine.com
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Environmental Monitoring Objectives: demonstrate that your choice of cleaners is robust and that your cleanrooms do not harbor high bacterial counts 264
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Environmental Monitoring Monitoring is performed on a routine basis Looking for both viable and non‐viable particulates Established ISO standards for non‐viable particulates Establish Alert and Action Levels Trending data
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Environmental Monitoring
Source: https://www.gotopac.com/art‐cr‐iso‐cleanroom‐classifications
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Environmental Monitoring Non‐Viable (Particulate) Monitoring Active Sampling Active monitoring indicates how many particles are in a m3 of air Measures different sized particles at .1 µm to 5.0 µm Performed in cleanrooms, BSCs, and LFUs
Source: https://www.climet.com
Source: https://encrypted‐tbn0.gstatic.com
Source: https://media.beckman.com
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Lab Environmental Monitoring
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Environment Monitoring – Non‐Viable (video)
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Environmental Monitoring Viable EM requires QC personnel to qualify the media Typically challenged with ≤ 100 cfu of various microbes including:
Aspergillus brasiliensis ATCC™ 16404 Bacillus subtilis ATCC™ 6633 Candida albicans ATCC™ 10231 Pseudomonas aeruginosa ATCC™ 9027 Staphylococcus aureus subsp. aureus ATCC™ 6538
Growth after 72 hours demonstrates the media can support microbial growth and can be used for EM monitoring activities.
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Environmental Monitoring Viable Monitoring Combination of active air sampling and passive monitoring Active monitoring indicates how many microbes are in a m3 of air Settling plates indicate how many microbes could settle onto a surface Touch plates indicate how many microbes are in approximately 25cm2 area
Source: https://www.rapidmicrobiology.com
Source: https://www.emdmillipore.com
Source: https://eagleanalytical.com
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Recommended limits for microbial contamination (EU) Recommended limits for microbial contamination Grade
Air sample cfu/m3
Settling plates (diam. 9 Contact plates (diameter Glove print 0mm cfu/4 hours) 55 mm) cfu/plate 5 fingers cfu/glove
A
<1
<1
<1
<1
B
10
5
5
5
C
100
50
25
‐
D
200
100
50
‐ Source: https://www.pda.org/docs
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Lab Environmental Monitoring
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Environment Monitoring – Air and Surface (Videos)
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Assessment
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Thank You! Contact Information: Cahil McGovern, Ph.D. (email: cahilmcgovern@uri.edu) Beth Zielinski‐Habershaw, Ph.D. (email: bzielinski@uri.edu) Malcolm Pluskal, Ph.D. (email: m.pluskal@verizon.net) Sharon McGuire, MS, (email: smcguire@uri.edu)
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Final Day Wrap Up and Evaluation
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