Aseptic Process Validation

Is a new FDA guidance imminent?

by Tom Spurgeon

What are the regulatory pressures facing aseptic process validation today and what will they be like over the next few years? An inquiry into existing literature and with current industry personnel reveals a corner of the pharmaceuticals industry driven by a lattice of suggested improvements, a constant hum of activity and improvements that fight to keep pace with general industry trends and emerging technology. Those working in aseptic processing validation must consistently look five years ahead and five years behind, at rules and informative processes and market realities, all of which play off one another like so many strings on a musical instrument. With an important FDA guidance revision just now beginning its long fade into routine and a brand new one described as imminent, aseptic processing and its regulatory outlook is at the forefront of pharma and biopharma business plans.

It's worth noting that the core guidance revisions for aseptic processing validation are still new. "The reason it's a hot area is that we had the aseptic processing guidance that was revised in 2004," said Hal Baseman, chief operating officer and a principal partner at Valsource.

Maurice Phelan, director of Pharmaceutical Technology, BioProcess Division at Millipore Corp., noted that newer statements are driving much of the attention: "The one thing that's gotten everybody interested, and sort of sparked a lot of interest in this subject over the last say year and a half, is the major statements by particularly the FDA about the need to change the way we manufacture sterile products."

Mr. Baseman added, "In September of 2004, there was a revision of the aseptic processing guidance. That resulted in a lot of discussion around validation of aseptic processing and things like that. It's always been a hot issue, an important issue, if you look at it from a risk management perspective. It's certainly a process that gathers a lot of attention."

Mr. Phelan sees the 2004 guidance as even more important in context. "I think it's the 2004 guidance, which was long awaited, but is also the strategic plan that the FDA has laid out, all of the concepts that are embodied in their GMPs for the 21st century initiative. All of the high-level sorts of concepts and aspirations that they have that are laid out in things like the Critical Path Initiative. And then there's the 2004 aseptic process guidance, when it's considered in the context of quality by design, design space concepts, all of the buzz in the industry around efficiency and manufacture, things like process analytical technologies -- when you consider all of those as contributors, then I think the buzz that's around aseptic processing and next generation manufacturing is a result of all of those together, and the context they have for whatever kind of manufacturing you do, whether it's biotech, or classical pharma-type manufacturing. It all depends on your interpretation on what it means to you."

The 2004 revision was the first major one since 1987, and therefore drew attention not just for the new standards it suggested, but for how the revision reflected modern industry practices. The result was a wave of attention to such issues that continues unabated. There are at least two major conferences this autumn that promise discussion of the subject, and specific classes on techniques involving aseptic processing and its validation that are filled weeks in advance. Mr. Phelan noted that there is genuine change reflected in the approach to process validation, within the hierarchy of validation.

He said, "Historically much of the body of work that would be called process validation wouldn't necessarily differentiate between that which was super-critical and that which was a required component but had variability that the process could tolerate. Intuitively the FDA is saying it's not just practical. Intuitively, if you've thought through a rationale that allows you to rank the criticality of unit operations in your process, then there should be a corresponding validation in your unit operations that's increasing in focus and scientific content as you go up the criticality scale. "I've heard an FDA inspector say, ‘Say what you're going to do. Prove that you can do it. And then when you get into manufacturing, do what you say you do.' That's a fairly straightforward statement for these guys to make."

In making its guidance revisions, the FDA gathers information from industry sources and then, once compiled, releases it back, causing a re-affirmation of the industry's best practices distinct, in its way, from standards the FDA might apply to drive companies into certain practices. At one meeting in 2002, the FDA's Advisory Committee For Pharmaceutical Science heard from several industry leaders and its own speakers on a variety of subjects related to aseptic process validation, including container-closure and sterile isolators. As Mr. Baseman put it, "Because we had an opportunity to comment extensively as the FDA allowed us to do [for the 2004 guidance], it became a reflection of what the industry was doing."

That give-and-take continues into the field. Said Mr. Phelan, "I heard this from the FDA as recently as last week: If you want to interact with them, and you're prepared to think about applying some of these next generation concepts, than they want to engage you." This is a change from times past, he noted. "Historically the FDA would have said, ‘Our door is open, and nobody's coming to talk to us. It's a one-way affair for us, and we have no option but assume a worst-case scenario. The only opportunity we have to share information is in the limited capacity of inspections or audits or reviews.' Now they're saying, ‘We have to change the way we do business. It's our view that you, the manufacturing community, need to look at how you manufacture and look at these types of areas.' Quality by design is the classic example of what they'd like to see.

"They've put programs into place," he added. "They have a pilot program that's gone on for the last 12 months for the review of new drug applications, where they've invited people to participate in basically a risk-based construct for the CMC sections in their new drug application."

The Guidance revision not only provides a platform for understanding the FDA's expectation and current industry practices, it also serves as a spur to science by offering up its own set of ways to approach certain problems while fostering from related organizations more up-to-the-minute, specific technical solutions.

With the FDA's more general efforts starting in 2001 to implement GMPs "for the 21st Century" -- itself two decades since the last similar effort -- came an emphasis on risk analysis. Risk analysis became the tool through which managers began to approach the validation of their aseptic processing techniques.

Mr. Baseman explained the general process as it has an impact on a facility's approach to their processing procedures: "Most biological contamination comes from people. So anything involving human intervention is going to be a riskier step. If we're doing an aseptic process test, let's say there's a step in there where somebody has to add a component manually, like a stopper. That becomes a riskier step. If we can eliminate that step by having some automated system to do that, then we eliminated and improve the process. That pushes us towards using isolators rather than conventional filling lines." The prioritization that comes with risk-management engenders a step-by-step vetting of the process validation. It puts emphasis on key points such as filtration, and then works its way backward to elements with less of a risk. As risk-management works its way to and then through those industry agents that have yet to fully embrace that approach, their use should become more and more routine.

This is just the way the FDA wants it, said Mr. Phelan. "Classically, validation exercises have been very, very document-heavy exercises. The FDA are now saying that we think there's a very practical approach to be taken in addressing all of the validation that needs to be done in a manufacturing process, assessing what the risks and/or overarching benefits are to putting so much effort into that enormous body of work, and then maybe thinking about a different way of justifying the amount of focus you put on in respect to validation, exercises based on their risk to your program."

Despite the fact that ideal sterilization technique is terminal, or heat-based, the market should drive more and more companies into aseptic processing. As most are quick to point out, terminal sterilization is a poor technique to apply to unstable products such as those represented by protein-based drugs. Aseptic processing places a specific emphasis on filtration as the last process performed to destroy organisms or contamination within a product. "Filtration would be where you would take the product, put it through a .2 micron filter and then fill it under very controlled conditions, in a clean room, perhaps in an isolator or perhaps in a conventional clean room but one with a lot of controls to keep the contamination out of the product," said Mr. Baseman. "Because there will be no subsequent step to destroy those organisms. That's why filtration is of interest related to aseptic processing."

With technology, market concerns and the introduction of new techniques and practices all driving interest in aseptic processing and its validation, one might think of the regulatory backbone as one of pressure and punishment. Actually, the opposite seems closer to the truth. Mr. Baseman praised the FDA for its ability to solicit commentary when preparing its guidances, both from individual players and major industry organizations like the Parenteral Drug Association (PDA). Not only does this give them a wider array of knowledge to use, the process settles industry players for whatever changes are to come. "I believe it's rare for the FDA to come out with something that's a big surprise," said Mr. Baseman. "For the most part what happens is that guidance gets issued that reflects what the FDA has been talking about and what the industry has been doing.

"I think there's an anticipation, but I don't think people are sitting there saying, ‘Maybe we shouldn't do any process validation this year because everything is going to change.' I don't think that's the case. The FDA has done a good job indicating where it's heading with this. They certainly put out some pretty good information in their initiative documents. There was a CPG that came out I think last year, but that CPG -- and that's their internal guidance document -- talked about what the agency would internally be looking for when it reviewed submissions. So if you read that, you kind of understood what the Agency is looking to do."

Groups like the PDA provide further support by issuing technical reports following guidances and standards, reports that provide a very specific way of meeting required standards, to be accepted, used or even refused, and make more clear the science of what's being done, away from purely regulatory motivations. For instance, PDA Technical Report #42 deals specifically and in what is described as a "practical" fashion with Process Validation in terms of protein manufacturing.

This system of multiple supports and reinforcements sets the stage for a revised guidance from the FDA for processing validation. Mr. Phelan characterized such revisions as "imminent." As to what that revision will entail, Mr. Baseman opined, "I think it may have something to do with new techniques. There's so much new technology that's coming out now, and I think it's important that the PDA weigh in on new technology, things down the road: new technologies for monitoring and so forth."

Mr. Phelan thinks the emphasis will be on the principles driving multiple solutions. "What I would expect is that it will contain all the intellectual components that one would classically associate with process validation and then it will have loaded on top of those good validation practices the concepts of design space, critical process parameters, risk-based decision-making and then practical validation approaches -- a rationale that says I understand what drives my process and I understand the critical parameters I need you to control and I need to validate.'"

As more companies are driven to work with drug forms that resist terminal sterilization, those that embrace GMPs and a risk-based outlook should find strong support in terms of aseptic process validation techniques, applied to steps ranging from filtration to use of isolators to air flow, that match the criticality of each phase to their overall function. Look for future guidance and technical papers to build on rather than replace the general outlook, at least until it becomes routine, as all former hot topics must sooner or later.

Tom Spurgeon is a contributing editor . He can be reached at tomspurgeon@yahoo.com

Pharmaceutical Sterility Testing

Essential things to know

By Steven Richter

Sterility testing of pharmaceutical articles is required during the sterilization validation process as well as for routine release testing. USP1 requirements employ sterility testing as an official test to determine suitability of a lot. An understanding of sterility testing is beneficial in terms of designing a validation process. The need to provide adequate and reliable sterility test data is an important quality assurance issue. Sterility testing is a very tedious and artful process that must be performed by trained and qualified laboratory personnel. The investigation of sterility test failures is a process that requires attention to environmental data as well as many other factors including training and sample difficulty.

This paper presents the general concepts and problems associated with sterility testing as well as the various testing methodologies. Most USP <71> sections are harmonized with the EP/JP.

Sterility testing is an essential part of every sterilization validation. Sterility testing is an extremely difficult process that must be designed and executed so as to eliminate false positive results. False positive results are generally due to laboratory contamination from the testing environment or technician error. The testing environment must be designed to meet the requirements of the United States Pharmacopeia (USP) in terms of viable microbial air and surface counts. Growth media used in sterility testing must be meticulously prepared and tested to ensure its ability to support microbial growth. Procedures for sampling, testing, and follow-up must be defined in the validation procedures.

Sampling Plans

The official test, the USP (Volume 30) recommends testing 40 units per production lot. A reprint of Table 2 "Minimum Quantity to be Used for Each Medium2" is on the next page. Some of the quantities are not harmonized with the EP/JP volumes.3

For combination products, the ISO 11137/111354 standards recommend various sterilization validation sampling plans based on lot size and validation method. In cases where small lots (>1000) are manufactured, the sampling size depends on lot size.

Environmental Concerns Related to Sterility Testing

The sterility test environment is described in USP General Informational Chapter <1211>. The environment should be as stringently controlled as an aseptic processing environment. An aseptic processing environment (clean room) is used to dispense sterile pharmaceuticals into presterilized containers. A clean room is generally a room that delivers laminar flow air which has been filtered through microbial retentive High Efficiency Particulate Air (HEPA) filters. The room is maintained under positive pressure and has specifications for room air changes per hour. An environment used for sterility testing should be similar in design to an aseptic processing environment; there should be an anteroom for gowning and a separate area for the actual sterility testing. The testing area should meet ISO Class 5 particulate control requirements (specified in USP chapter (1116)). Sterility testing should not be carried out under a laminar flow hood located within a room that is not maintained as ISO Class 5. Along with particulate testing in the environment, the laboratory must test for viable bacterial and fungal organisms ubiquitous to it. The sterility test technician must be suitably gowned in sterile garments that prevent microbial shedding into the room. The room should be validated in terms of particulate and microbial levels. The laboratory must have a validation and training program for gowning and sterility testing.

Our validation programs require that technicians consecutively test 40 simulated samples for both membrane filtration and direct immersion methods without a false positive test result under less than ideal environmental conditions. Isolator technology is utilized to create a sterile environment for one to test pharmaceutical articles. The validation required to qualify an isolator is extensive. The isolators are generally sterilized using chemical sterilization.

Many issues surround the robustness of the sterilization process. Qualifying and maintaining an isolator system for sterility testing may require extensive work. In testing pharmaceutical articles in a closed system such as Steritest^TM, an isolator may not be the best cost approach to the environmental concerns. Most environmental concerns can be obviated by standard aseptic processing GMP's.5

Methodologies

The United States Pharmacopeia is a compilation of validated methods and official monographs for pharmaceuticals and medical devices. IT is broken down into the following sections: Monographs, General Informational Chapters, and General Requirements. General Informational Chapters <1000> series are not legal requirements. The Sterility Test (USP Section <71>) is categorized under General Requirements and is therefore a legal requirement.

For combination products, the ISO radiation sterilization microbial methods (11737-2 1998)6 describes a sterility test which is a modification for the USP method. This test is specific for the detection of aerobic organisms that have been exposed to sub-lethal sterilization cycles. This ISO sterility test method is recommended for the validation of both gamma and electron beam sterilization processes.

The method of choice for EO7 sterilized products is the official USP <71> procedure.

Processes

Prior to actual sterility testing, it is prudent to send an example sample to the testing laboratory so the laboratory can determine the appropriate testing procedure. Each product should have a unique procedural specification for testing. The procedure should be very specific in terms of which items (or vials/syringes) to test. The procedure must indicate the Sample Item Portion (SIP). The Sample Item Portion is the percentage of the complete product tested. Since medical devices come in all shapes and sizes, it is very difficult to test large and cumbersome medical devices in their entirety. Therefore, the test laboratory will determine a Sample Item Portion which is a portion of the sample expressed in fractional terms (i.e. 0.1 for 10% of the sample).

This number is used in gamma and electron beam dose setting methods. The SIP portion should be validated by sterility testing.

Combination products have unique challenges. A combination product is defined as one that has a drug component with medical device. For example, a drug coated stent. The agency's Office of Combination Products (OCP) would determine which regulatory branch (CDRH, CDER or CBER) is officiating the product. Official USP sterility testing of combination products is required for all sterile drug products. The drug product component applied aseptically creates the largest challenge to laboratory personnel. Biologics must be aseptically processed and cannot be terminally sterilized. In the near future, we will see more biologics that are combination products. Combination products sterilized by radiation are generally handled as medical devices following the ISO 11137 standard. For the most part, pharmaceutical GMPs would take precedent over 820 QSR8 requirements with all combination products. The more robust GMP9 requirement would assure reduced bioburden counts and consistent microbial populations during manufacturing.

The USP <71> Sterility Test contains two qualifying assays which must be performed prior to sterility testing. They are the "Suitability Test" (Growth Promotion Test) and the "Validation Test" (Bacteriostasis and Fungistasis Test).

The Suitability Test is used to confirm that each lot of growth media used in the sterility test procedure will support the growth of fewer than 100 viable microorganisms. If the media cannot support the growth of the indicator organisms, then the test fails. Secondly, a portion of each media lot must be incubated and assessed for sterility according to the incubation parameters (time, temperature) established by the method. If the media is found to be non-sterile, then the test fails.

The Validation Test is used to determine if the test sample will inhibit the growth of microorganisms in the test media. Stasis, in terms of microbiology, is defined as the inability of a microorganism to grow and proliferate in microbiological media. Media that is bacteriostatic does not necessarily kill bacteria; it simply may retard bacterial growth and proliferation. The Validation Test must be performed on each product prior to and/or during sterility testing. This test determines if the media volumes are valid for the particular product. Some medical products contain bacteriostatic and fungistatic compounds that may require special procedures and special media for testing. This test is similar to the Suitability Test described above, however, the product sample is placed in the media along with the microorganisms. Microbial growth in the presence of the test samples is compared to controls without test samples. If microbial growth is present in the sample and control containers, then the test is valid. The next step is to proceed to actual sterility testing. Suitability, validation and sterility tests can be performed simultaneously.

The USP describes three general methods for sterility testing: 1) Membrane Filtration, 2) Direct Transfer (Product Immersion); and 3) Product Flush.

Membrane Filtration Sterility Testing

The Membrane Filtration Sterility Test is the method of choice for pharmaceutical products. It is not the method of choice for medical devices; the FDA may question the rationale behind using the membrane filtration test over the direct transfer test for devices. An appropriate use of this test is for devices that contain a preservative and are bacteriostatic and/or fungistatic under the direct transfer method. With membrane filtration, the concept is that the microorganisms will collect onto the surface of a 0.45 micron pore size filter. This filter is segmented and transferred to appropriate media. The test media are fluid thioglycollate medium (FTM) and soybean casein digest medium (SCDM). FTM is selected based upon its ability to support the growth of anaerobic and aerobic microorganisms. SCDM is selected based upon its ability to support a wide range of aerobic bacteria and fungi (i.e. yeasts and molds). The incubation time is 14 days. Since there are many manipulations required for membrane filtration medical device sterility testing, the propensity for laboratory contamination is high. Therefore, in an open system, more sterility failures are expected when using this method. A closed system is recommended for drugs and small devices or combination products. Most pharmaceutical articles are tested using a closed system. In closed systems, the propensity for extrinsic contamination is very low.

Direct Transfer Sterility Testing

Combination products: This method is the method of choice for medical devices because the device is in direct contact with test media throughout the incubation period. Viable microorganisms that may be in or on a product after faulty/inadequate sterilization have an ideal environment within which to grow and proliferate. This is especially true with damaged microorganisms where the damage is due to a sub-lethal sterilization process. All microorganisms have biological repair mechanisms that can take advantage of environmental conditions conducive to growth. The direct transfer method benefits these damaged microorganisms. The entire product should be immersed in test fluid. With large devices, patient contact areas should be immersed. Large catheters can be syringe filled with test media prior to immersion. Cutting catheter samples to allow for complete immersion is the method of choice.

The USP authors understand that appropriate modifications are required due to the size and shape of the test samples. The method requires that the product be transferred to separate containers of both FTM and SCDM. The product is aseptically cut, or transferred whole, into the media containers. The test article should be completely immersed in the test media. The USP limits the media volume to 2500 ml. After transferring, the samples are incubated for 14 days.

Product Flush Sterility Testing

Combination products: The product flush sterility test is reserved for products that have hollow tubes such as transfusion and infusion assemblies where immersion is impractical and where the fluid pathway is labeled as sterile. This method is easy to perform and requires a modification of the FTM media for small lumen devices. The products are flushed with fluid D and the eluate is membrane filtered and placed into FTM and SCDM. This method is not generally used.

Bulk Drug Products / Biologics and Pharmaceuticals

Bulk Pharmaceuticals (APIs) are tested for sterility per USP 71 prior to release to the manufacturing processes.

Bulk Biologics are tested according to 21 CFR 610.12 for sterility testing. This method requires one media (FTM). The sample test sizes are listed in the document. Volumes are no less than 10 ml.10

Interpretation of Sterility Test Results

The technician must be trained in the method of detecting growth during the incubation period. Growth is determined by viewing the media, which is generally clear and transparent, against a light source. Turbid (cloudy) areas in the media are indicative of microbial growth. Once growth is detected, the suspect vessel is tested to confirm that the turbidity present is due to microorganisms and not due to disintegration of the sample; sometimes samples produce turbidity because of particulate shedding or chemical reactions with the media. Once a suspect container has been tested, it should be returned to the incubator for the remainder of the incubation period. Samples that render the media turbid are transferred on Day 14 of the test and incubated for four days. Growth positive samples require further processing such as identification and storage.

Sterility Test Failure Investigation

For every positive sterility test (OOS), the laboratory should perform an OOS investigation to determine the validity of the positive growth. This investigation encompasses the following items:

1. clean room environmental test (EER) data;
2. media sterilization records;
3. technician training records;
4. the relative difficulty of the test procedure;
5. control data (open and closed media controls);
6. technician sampling data (microbial counts on gloves and/or garments post testing).

The USP allows for a re-test of the product if persuasive evidence exists to show that the cause of the initial sterility failure was induced by the laboratory. Identification and speciation of the isolate(s) is a significant contributing factor to the final decision. If the First Stage sterility test can be invalidated by the laboratory, then the USP allows for Second Stage sterility testing. Second Stage sterility testing requires double the original number of samples tested. The Second Stage test can be repeated if evidence exists invalidating the test due to a laboratory error as above.

A detailed investigation may uncover circumstantial evidence to support a final decision. It is recommended that sterilization cycle data, environmental data, and bioburden data be reviewed prior to making any decision to release product.

It is recommended that medical device manufacturers qualify the test procedure with non-sterile samples.

The probability of a false positive can be calculated using John Lee's formula.11 The formula is based upon sample container diameter, amount of time container is left open and the room particulate count.

Sterility testing requires high levels of control with regards to GMPs, Good Laboratory Practices12, environment (aseptic clean room ISO class 5 or better), and employee practices. It is essential that meticulous technique be employed in the practice of sterility testing. Sterility testing is an integral part of sterilization validation as well as a routine quality control. Generally, false positive results are uncommon in testing drug products using a closed system. Combination products have challenges that should be planned into a robust QA program.

References

1. The United States Pharmacopeia, 30th Revision, The United States Pharmacopeial Convention: 2008
2. USP 30 Table 2 Minimum Quantity to be Used for Each Medium
3. USP 30 Table 3: Minimum Number of Articles to be Tested in Relation to the Number of Articles in the Batch
4. ISO 11137 Sterilization of health care products – Radiation – Part 2 2006: Establishing the sterilization dose
5. FDA Guidelines 2004 "Guidance for Industry Sterile Drug Products by Aseptic Processing, Current Good Manufacturing Practices," September, 2004
6. ISO 11737 ANSI/AAMI/ISO 11737-2 1998 – Sterilization of Medical Devices – Microbiological Methods – Part 2, Tests of Sterility Performed in the Validation of a Sterilization Process
7. ISO 11135 1994 Medical Devices Validation and Routine Control of Ethylene Oxide Sterilization
8. Code of Federal Regulations Title 21/Chapter I/Part 820, "Quality Systems Requirements: General," 2006
9. GMPs CFR 201 Title 21 2006
10. 21 CFR Part 610.12 Bulk Biologics
11. Lee, John Y. "Investigation Sterility Test Failures" Pharmaceutical Technology, February 1990
12. Code of Federal Regulations Title 21/Chapter I/Part 58, "Good Laboratory Practice for Nonclinical Laboratory Studies," 2006

Thermal Validation in the Pharmaceutical Industry

An argument against the use of thermocouples

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The pharmaceutical industry is a highly regulated environment based on research, evidence, record-keeping, and validation. The term "thermal validation" is the process of validating / qualifying equipment and storage facilities to prove that they will create and maintain the temperatures they are designed for.

For those responsible, choosing the right temperature validation tool is decision #1 - and making that choice requires a thorough understanding of different sensor types. This paper will specifically focus on two common sensors: thermocouples and thermistors (see table below).

With nearly a decade of experience using both thermocouples and thermistors, Veriteq Instruments knows the advantages and disadvantages of each sensor, and will discuss them in this article as they relate to data logging in the pharmaceutical industry. This paper will also include specific references to Veriteq data loggers, which utilize internal thermistors. But first, a brief definition of thermocouples and thermistors:

• A thermocouple is made of two dissimilar metals in contact with each other. The thermocouple works by generating a small voltage signal proportional to the temperature difference between the junctions of two metals.
• In contrast, a thermistor is a resistive device made up of metal oxides that are formed into a bead and encapsulated in epoxy or glass. As temperature changes, so does resistance, causing a large voltage drop. Both sensors are quite small and normally encased in a protective shell, stainless probe, or wire coating, meaning that they may look very similar to the end-user.

  

	Thermocouple	Thermistor
Temp. Range	-270 to 1800°C (-454 to 3272°F)	-86 to 150°C (-123 to 302°F)
Sensitivity	Low	High
Stability	Low	High
*Time-savings	Lengthy set-up	Minimal set-up
*Sources of Error	Many	Few
*Accuracy	Low	High
Ideal Applications	High temperature oven profiling, Cryogenic freezing	Warehouse monitoring, Stability testing, Chamber qualification, Cooler and Freezer, Monitoring, Lab monitoring, Cold Chain monitoring.

* This comparison looks at a total data logging system, and not just the sensor.

Temperature Range

Thermocouples offer the widest range of measuring capabilities, which admittedly makes them a suitable choice for extreme temperature applications such as oven profiling and cryogenic freezing.

However, in the range of -86 to 150°C (-123°F to 302°F), thermistors become an option, and for most applications they are the better choice. Thermistors are primary sensors, meaning that they operate independently, without the need for a second reference sensor. In fact other systems, including thermocouple systems, often use thermistors as their reference sensor.

It should be noted that the stated temperature range of -80 to 150°C (-123°F to 302°F) is just for the thermistor itself, and not for an enclosed Veriteq data logger. Veriteq data loggers are designed to withstand the range of -86 to 85°C (-123°F to 185°F) meaning that the loggers themselves can be placed in the temperature environment and left there. This makes them an ideal solution for chamber qualifications, stability testing, warehouse, cooler and freezer monitoring.

Veriteq's solution for the higher range of 85°C to 150°C (185°F to 302°F) requires an external thermistor probe that allows the connected data logger to remains outside the high temperature environment.

Sensitivity

The term sensitivity refers to the size of signal received in response to a temperature change, and is an important component of sensor accuracy. Thermistors are highly sensitive; in fact the name thermistor evolved from the phrase "thermally sensitive resistor". Stuart Ball, an electrical engineer and author for embedded.com writes that "of all passive temperature measurement sensors, thermistors have the highest sensitivity."

In comparing thermistors with thermocouples, Stuart goes on to say: "The voltage produced by a thermocouple is very small, typically only a few millivolts. A type K thermocouple changes only about 40 microvolts per 1°C (1.8°F) change in temperature." With such a small voltage to measure, it becomes difficult to distinguish an actual temperature change from noise. Enercorp Instruments Ltd., a provider of thermocouples and thermistors, speaks directly to this issue:

"The voltage produced is very small and amounts to only a few microvolts per degree Celsius. Thermocouples are therefore not generally used within the range of -30 to 50°C (-22 to 122°F)".

The graphs below are a visual representation of the increased sensitivity that a thermistor based system (such as a Veriteq data logger) detects as compared to a thermocouple system.

Stability

Thermistors are very stable, which makes them ideal for portable applications such as warehouse and chamber qualifications. For example, Veriteq data loggers can be moved frequently without calibration, and still maintain an accuracy of +/- 0.15°C (+/-0.27°F).

To prove the point, Veriteq recently checked the calibration of 106 data loggers after a year of use in the field. Each logger was checked at the following calibration points: -20°C, 25°C, and 70°C. The results were impressive, showing less than 1% of the points to have any excess drift. Still, Veriteq recommends that data loggers are re-calibrated on a yearly basis.

Thermocouples, on the other hand, are known for low stability, which is why a pre-cal / post-cal is required with every use.

Time-savings

A Veriteq data logger is a system in itself, and one that is easy to use. Each data logger, containing a thermistor, is simply set to the desired sampling frequency and then placed in the monitoring location. Following the test period, the data is downloaded via a PC or PDA. The system is very straightforward and doesn't require any stringing of wires - the result is a significant time savings.

In contrast, a thermocouple based set-up can be quite time consuming, especially for high-accuracy applications requiring a pre and post-calibration. For example, qualifying a chamber with a thermocouple system involves first putting all sensor ends (i.e. the hot junctions) inside a calibration unit and going through the pre-calibration process. Following a successful calibration, the thermocouples are strung from the central data logging unit, to the chamber, through a door seal, and then taped into various positions. Care must be taken to keep a good seal on the door while minimizing damage to the thermocouple wire. Only then can the data collection begin. And when that is complete, all thermocouple sensors must still be moved to the calibration unit for post-calibration. Finally, it is not uncommon for thermocouples to fail the post-calibration, meaning that the whole process may need to be repeated.

Sources of Error

Being a self-contained unit means that Veriteq data loggers have less error sources to deal with - there are no wiring errors, no cold junction errors, and no errors associated with in-field calibration (see table below).

	Thermocouple System	Veriteq Thermistor System
Physical damage to sensor	"Cold working" degrades thermocouple wires as they are repeatedly bent, stepped on, or shut in chamber doors.	There is minimal risk because the thermistor sensor is protected inside the data logger
Non homogeneity Consistency of thermocouple wire and the environment it runs through	Always present to some extent	N/A
Cold Junction reference error Temperature deviation between cold junction reference point and the actual cold junction; includes accuracy of cold junction sensor	The single largest source of error	N/A
Pre & post calibration errors: Reference transfer calibration error; traceable temperature standard; environmental stability; movement of sensors	In-field calibration introduces many sources of error	Pre & post calibration is not required
Operator Error	High level of knowledge required to minimize errors	Less risk as the system is relatively simple
Analog to Digital conversion	Minor	Minor

In contrast, thermocouple systems have numerous sources of error, the most significant being the cold junction reference error. Goran Bringert, of Kaye Instruments, states the following:

"A change in ambient temperature is the most significant source or error in thermocouple measuring systems, particularly multi-channel systems with internal cold junction references"

Accuracy

High accuracy is critical for temperature validations because of the 4:1 rule, which recommends that instruments be at least four times as accurate as the parameter being measured/validated. Therefore, Veriteq data loggers, with their accuracy of +/- 0.15°C (+/-.27°F), can be used to monitor/validate parameters as tight as +/- 0.60°C (+/-1.1°F).

As for thermocouple based systems, a leading provider claims to have a total system accuracy of +/- 0.28°C (+/-0.5°F). While this may be true from a theoretical point of view, it would require having optimal conditions available. Others in the industry believe that +/- 1 to 2°C (+/- 1.8 to 3.6°F) is a more realistic accuracy for such a system, meaning that it could be used to validate parameter specifications of +/- 4 to 8°C (+/-7.2 to 14.4°F), applying the 4:1 rule. In any event, very few people dispute the fact that thermistors are more accurate than thermocouples.

Conclusion

When choosing a system for performing thermal validations, the first question asked should be "what kind of sensor is being used?"

Thermocouple sensors should be avoided because they involve a lengthy set-up, numerous error sources, and marginal accuracy. It would be best to restrict thermocouple systems to applications involving very high or very low temperatures, simply because there are no other choices available at those extremes.

In contrast, thermistor sensors are ideally suited to high accuracy monitoring in the range of -86° to 150°C (-123°F to 302°F). The Veriteq thermistor based system is highly sensitive, stable, accurate and easy to use. In addition, it eliminates the many error sources associated with thermocouple systems, and allows for a much quicker set-up time. In short, you save time, experience less hassle, and obtain high-accuracy results.

Is Your Relative Humidity Monitoring System Safe?

In the pharmaceutical industry, relative humidity (RH) must be carefully controlled to ensure suitable manufacturing and storage environments and to assure proper stability testing. If the RH rises or falls above pre-established parameters, it can jeopardize product quality, derail FDA submissions, increase liability and damage a company' s reputation. And while many companies rely on RH regulating control systems to monitor and control humidity within their facilities, few realize just how sensitive and prone to distortion RH sensors can be.

Factors That Affect Sensor Functionality

RH sensors are "air breathers." Like tiny sponges, they "absorb" water vapor from the air. To function properly, RH sensors must maintain intimate contact with the environment. Unfortunately, this exposure leaves sensors vulnerable to airborne contaminants such as chemicals and cleaners, which can coat or permanently damage a sensor's surface, prevent it from properly absorbing water vapor and ultimately distort its signal.

Even simple condensation can affect an RH sensor's accuracy. If the door to a high humidity environment is opened, for example, condensation may form on the RH sensor inside. Long after the RH reading appears normal, the sensor can remain wet internally causing an offset in value and it may need to be removed and dried before it can once again provide accurate readings.

To ensure RH remains within a given range, many companies install RH system alarms. However, as I'll demonstrate below, these alarms provide a false sense of security. In reality, RH sensors can drift -- and RH can stray well outside pre-established parameters -- without any notification from the alarm system.

RH control systems work by measuring the current RH, comparing it against a desired setpoint and automatically increasing or decreasing humidity as necessary to achieve and maintain the setpoint. RH sensors convey information via electrical signals that are proportionate to the amount of RH detected. For every 10 percentage points that humidity varies, for example, the sensor might send a 1-volt signal. RH recorders, displays and system alarms work by monitoring these same electrical signals. The alarm system will alert users if they stray outside a pre-defined range (e.g. 35%-45%, or 3.5V-4.5V).

If an RH sensor has been damaged or contaminated, it might send a signal of 4V, indicating 40% humidity – and the system display would reflect this – when in reality the relative humidity might be just 38%. As this sensor drifts over time, it may continue sending a 4V signal, when RH is just 36%, then 34%, and so on until the RH is well outside the pre-defined range of 35%-45%. And yet, because the RH alarm system relies on the sensor signal, and the signal remains at 4V, the alarm system will not be activated and the system display and recorder will look normal.

Factors That Affect Sensor Functionality

How can your company protect itself from the challenges inherent in RH sensors? By incorporating redundancy and using two RH sensors – one to regulate the RH and a second, independent sensor to monitor the system. The second sensor will verify the results from the primary sensor and highlight any irregularities or discrepancies. And, while it' s technically possible for both sensors to become distorted, the likelihood that both will drift at exactly the same rate, and exactly the same time, is miniscule. As long as there's variation between the two, you' ll know a potential problem exists.

In addition to verifying the results of your primary RH sensor, a secondary sensor can provide continuous monitoring during primary system failures. The secondary sensor will supply a valuable record of RH levels throughout the system failure, enabling you to identify potential problems that may have occurred as a result.

To maximize the benefit from your secondary sensor system, choose one with an extended battery life. If your primary system is knocked out due to power failure, your secondary system may need to function on battery power for an extended period of time. Some sensors have batteries that last 10 years while others are unlikely to last through a long weekend.

To minimize malfunctions and down time, choose a secondary RH system that's easy to use, with a minimum number of moving parts. Chart recorder's pens, for example, can run out of ink and recorder paper must be replaced regularly. A better option might be a data logger, which is self-contained, has no moving parts and can be installed in minutes.

For the most accurate results, place sensors as far apart as possible within the monitored environment. This way, if contamination or condensation occurs in one area of the space, the chance of both sensors being affected in the same way is greatly reduced. Also, because temperature variations can have a significant impact on RH, the RH in an environment is much less uniform than you might think. In a stability chamber operating at 40°C and 75% RH, for example, 1°C of nonuniformity will cause a 4% variation in RH. While the amount of water in the air may remain close to constant, the RH may not. Positioning sensors at multiple monitoring points gives you a much more accurate idea of what's happening throughout the environment.

While risk reduction through redundancy is common in many other process control applications, the pharmaceutical industry has been slow to adopt this practice. This may be due in part to price – it used to cost several thousand dollars to set up a second RH sensor system. Today, however, when a complete, self-contained secondary monitoring system can be purchased for around a third as much, there's simply no excuse for not protecting your company' s operations, products, clients and reputation by building redundancy into RH regulating systems.

Written by Kevin Bull.

Originally published in the March 2006 edition of Pharmaceutical Processing Magazine.

Catching the Drift: What the Specifications of Your Humidity Measurement System Might be Missing

One of the hardest parameters to accurately measure, relative humidity is a pivotal factor across a broad spectrum of industries and often entails the potential to impact critical applications and public safety. In calibration, stability testing, or quality assurance processes, the intrinsic uncertainty of humidity measurement can be a major source of unnecessary cost, skewed data, and lost revenues.

Product data sheets for all relative humidity measuring devices must be scrutinized to ensure the system is sufficient for the application it will be used in. Basic knowledge of how these devices function will prove that often, critical information that is not provided by a manufacturer can be more revealing than what is.

Introduction

Understanding how RH measuring devices function and how those functions are commonly represented in product specifications can help with selecting the right system.

Knowing what to look for in product specifications can also initiate incisive questioning of manufacturers about the accuracy of their humidity measuring systems.

Fact: All Humidity Sensors Drift

It's an immutable law of RH measurement. Sensors drift for the simple reason that they are air breathers. Unlike temperature sensors, the internal structure of the humidity sensor must be in direct contact with the environment, which is constantly changing temperature and contains airborne contaminants. Both temperature and contaminants significantly affect the accuracy of any RH sensor. This is why, even if the calibration process were perfect (it isn't), once exposed to the real world, the measurement accuracy inevitably degrades.

RH Accuracy: Initial vs. One Year Later

There are two key accuracy values that must be considered when looking at any RH measuring device's product specifications. The first is Initial Accuracy; the other is One Year Accuracy.

Initial Accuracy is the device's accuracy when first deployed, fresh from calibration. This amount should include all known uncertainties:

• Calibration Uncertainty
• Temperature Effect & Mathematical Fit
• Hysteresis
• Measurement Resolution

One Year Accuracy is the accuracy of the device after a year of normal use — the typical interval between calibrations. Although One Year Accuracy is a critical value, it is usually excluded from product specifications.

The reason that the One Year Accuracy is such a key piece of information is that all data gathered with an instrument since its last calibration is based solely on its accuracy when it's re-calibrated.

For example, if your RH measurement device is found out-of-spec when re-calibrated, you will be faced with some hard choices. What products or tests were affected and to what extent?

Creating Headroom

Veriteq Instruments states the accuracy of their RH measuring devices after a year of typical use and over a wide temperature range on their spec sheets. The question is: why is the inclusion of these values on product specifications so rare within the industry?

To answer this question, it's vital to understand what determines sensor accuracy. There are three main elements:

• Sensor characteristics
• Calibration
• Sensor Measurement System (Electronics)

While Veriteq uses the best RH sensor available, as already stated: all RH sensors drift. To maximize overall accuracy, it is crucial to reduce errors that occur in the Calibration process and Sensor Measurement System.

This creates what Veriteq calls "Sensor Drift Headroom". In terms of instrument accuracy, "Headroom" is created by achieving optimal accuracy in Calibration and the Sensor Measurement System, thereby accommodating the impact of drift. Headroom in effect anticipates the drift by reducing or virtually eliminating all other sources of error.

Calibration Uncertainty

All humidity calibration chambers have an associated uncertainty, a major source of which is temperature non-uniformity. This must be factored into a measuring device's accuracy specification.

Before humidity calibration, Veriteq performs a high-accuracy temperature calibration on every data recorder. Each recorder's measured temperature is then able to compensate for chamber non-uniformity during RH calibration — greatly reducing this source of error.

Temperature Effect & Mathematical Fit

Most RH measuring devices are calibrated to measure at one specific temperature (typically 25ºC). But, unless the device will only be used to measure humidity at that temperature, there can be significant temperature-related inaccuracies.

To solve this, there are 256 tables residing in the memory of every Veriteq humidity data recorder. These tables correlate humidity measurement over a wide range of calibrated temperatures. No two data recorders have the same set of tables because each set is calibrated to the unique components of every recorder.

Unlike other humidity recorders, Veriteq's is an 'intelligent' device, because it contains explicit information on how to measure humidity over a wide temperature range. This is particularly important in the case of ICH (stability) applications.

Hysteresis

Hysteresis is the tendency of measuring devices to not return completely to their original state after a change has been measured. When measuring relative humidity, it can be a major source of error.

Unfortunately, too few data sheets include hysteresis as a factor in their accuracy values. If it appears at all, it's often de-emphasized by being placed far apart from the total accuracy specification. Hysteresis unmentioned or disconnected from an accuracy value should be considered product data misrepresentation.

Measurement Resolution

Resolution is simply the smallest measurable increment that the device can detect. Veriteq uses a 12-bit high-resolution system that detects changes of as small as 0.05%RH.

Veriteq's Sensor Measurement System

A significant element that affects a device's accuracy is its electronic measurement system. Electronics systems are greatly impacted by temperature, which in turn affects overall measurement accuracy.

Veriteq's solution was to create a proprietary electronic system that has proved to be ultra-stable over wide temperature ranges. This new approach —based on a synchronous bridge measurement system — features low power and unmatched stability.

For an in-depth description of Veriteq's Sensor Measurement System, see Methods of Accurately Measuring Capacitive RH Sensors

Conclusion

Product specifications, often one of the only ways decision makers can select a suitable system, must be explicit, easy-to-understand, and straightforward.

All of the known influences and sources of error — calibration uncertainty, temperature effect, measurement resolution, and hysteresis — should be included in the accuracy value stated on any data sheet. If these values are not mentioned on a product data sheet, have they been included in that product's stated accuracy?

Manufacturers confronted with their own out-of-spec devices upon re-calibration, can always blame drift — rather than lack of diligence in eliminating sources of error.

About Veriteq

Since 1994, Veriteq Instruments has been innovating new methods to measure RH and temperature and providing accessible, validatable, and accurate data for both regulated and non-FDA/GxP industrial use.

Veriteq works with a wide variety of industries and applications; from pharmaceutical companies, biotech and calibration laboratories, aerospace engineering facilities, to storage facilities for sensitive products.

Veriteq's system features an industry leading 10-year battery life and all products come with comprehensive specifications for Initial and One Year Accuracies. Veriteq also provides software, monitoring and alarming solutions.

In essence, their approach is better technology, increased accuracy, and total transparency in product information. Veriteq's commitment to accuracy is evident in the solutions they create, as well as their product specifications, which are industry leading in depth and integrity.

Thermal Validation: Matching Tool to Task

Download the complete article.

Synopsis:

This peer-reviewed article explains how the proven stability of Veriteq's thermistor-based data loggers is the key to eliminating pre- and post-calibrations, which allows for unprecedented accuracy and efficiency in thermal validation projects.

Evidence That Stable Sensors Eliminate Pre- & Post-Calibration

As outlined in the article, our A2LA accredited calibration laboratory performed 2,427 routine service calibrations on Veriteq data loggers that had been in field use for 10 to 14 months. Of these devices, 99.7% were returned for calibration well within the original accuracy specifications. Of the eight that were found Out of Specification (OOS), none were out by more than 0.12ºC, and the average OOS value was 0.036ºC.

These results indicate that, with the Veriteq Validation System, skipping pre- and post-calibrations is not reckless practice. The stability of the data loggers allows for a more efficient and accurate validation method. In addition, the reduced set-up and deployment time of our system, along with little or no operational downtime that normally accompanies validating with thermocouple-based sytems, reduces many of the high costs associated with validation.

The article was published in the winter 2008 issue of the Journal of Validation Technology.

Method Development of Swab Sampling for Cleaning Validation of a Residual API

• Read more

cross contamination with active ingredients is a real concern. The Code of Federal Regulations (CFR) states that "Equipment and utensils shall be cleaned, maintained, and sanitized at appropriate intervals to prevent malfunctions or contamination that would alter the safety, identity, strength, quality, or purity of the drug product beyond the official, or other established requirements" (1). Cleaning validation is required in the pharmaceutical field to avoid potential clinically significant synergistic interactions between armacologically active chemicals (2). Since the issuance of the US Food and Drug Administration's "Guide to Inspection of Validation of Cleaning Process" in July 1993 (3), cleaning validations have received increasing attention.Validation is required not only for manufacturing sites, but also for the sampling- filling suite in research and development.

Author(s):

Pei Yang, et al

Journal:

Pharmaceutical Technology, Jan 2, 2005